- Email: [email protected]
Mycobacterium abscessus ESX-3 plays an important role in host inflammatory and pathological responses during infection
Accepted Manuscript Mycobacterium abscessus ESX-3 plays an important role in host inflammatory and pathological responses during infection Yi Sak Kim, Chul-Su Yang, Loi T. Nguyen, Jin Kyung Kim, Hyo Sun Jin, Jin ho Choe, Soo Yeon Kim, Hye-Mi Lee, Mingyu Jung, Jin-Man Kim, Myung Hee Kim, EunKyeong Jo, Ji-Chan Jang PII:
S1286-4579(16)30123-X
DOI:
10.1016/j.micinf.2016.09.001
Reference:
MICINF 4426
To appear in:
Microbes and Infection
Received Date: 25 February 2016 Revised Date:
2 August 2016
Accepted Date: 5 September 2016
Please cite this article as: Y.S. Kim, C.-S. Yang, L.T. Nguyen, J.K. Kim, H.S. Jin, J.h. Choe, S.Y. Kim, H.-M. Lee, M. Jung, J.-M. Kim, M.H. Kim, E.-K. Jo, J.-C. Jang, Mycobacterium abscessus ESX-3 plays an important role in host inflammatory and pathological responses during infection, Microbes and Infection (2016), doi: 10.1016/j.micinf.2016.09.001. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
ACCEPTED MANUSCRIPT 1
Mycobacterium abscessus ESX-3 plays an important role in host inflammatory
2
and pathological responses during infection
3
Yi Sak Kim,1,3† Chul-Su Yang,4† Loi T. Nguyen,5 Jin Kyung Kim,1,3 Hyo Sun Jin,1,3 Jin
5
ho Choe,1,3 Soo Yeon Kim,1,3 Hye-Mi Lee,1,3 Mingyu Jung,2,3 Jin-Man Kim,2,3 Myung Hee
6
Kim,5 Eun-Kyeong Jo,1,3 and Ji-Chan Jang1,3,6*
7
RI PT
4
1
Department of Microbiology and 2Pathology, 3Department of Medical Science, College of
9
Medicine, Chungnam National University, Daejeon 301-747, Korea.
SC
8
4
Department of
Molecular and Life Science, Hanyang University, Ansan 426-791, Korea. 5Infection and
11
Immunity Research Center, Korea Research Institute of Bioscience and Biotechnology,
12
Daejeon 305-806, Korea. 6Molecular Mechanism of Antibiotics, Division of Life Science,
13
Research Institute of Life Science, Gyeongsang National University, Jinju, Gyeongnam,
14
Korea
18 19 20 21
TE D
17
EP
16
AC C
15
M AN U
10
*For correspondence. E-mail: [email protected];
22
Tel. (+82) (0)55 772 1368
23
† Both authors contributed equally to this work.
24
ACCEPTED MANUSCRIPT 25
Abstract Mycobacterial ESX systems are often related to pathogenesis during infection.
27
However, little is known about the function of ESX systems of Mycobacterium abscessus
28
(Mab). This study focuses on the Mab ESX-3 cluster, which contains major genes such as
29
esxH (Rv0288, low molecular weight protein antigen 7; CFP-7) and esxG (Rv0287, ESAT-6
30
like protein). An esx-3 (MAB 2224c-2234c)-deletional mutant of Mab (∆esx) was constructed
31
and used to infect murine and human macrophages. We then investigated whether Mab
32
∆esx modulated innate host immune responses in macrophages. Mab ∆esx infection
33
resulted in less pathological and inflammatory responses. Additionally, ∆esx resulted in
34
significantly decreased activation of inflammatory signaling and cytokine production in
35
macrophages compared to WT. Moreover, recombinant EsxG▪EsxH (rEsxGH) proteins
36
encoded by the ESX-3 region showed synergistic enhancement of inflammatory cytokine
37
generation in macrophages infected with ∆esx. Taken together, our data suggest that Mab
38
ESX-3 plays an important role in inflammatory and pathological responses during Mab
39
infection.
42 43 44 45
SC
M AN U
TE D EP
41
Keywords : Mycobacterium abscessus; ESX-3; host inflammation
AC C
40
RI PT
26
ACCEPTED MANUSCRIPT 46
1. Introduction Mycobacterium abscessus (hereafter referred to as Mab) is the most pathogenic strain
48
of the Mab complex, a group of rapidly growing non-tuberculous mycobacteria (NTM) and a
49
pathogenic mycobacterium [1]. Mab is commonly associated with a wide spectrum of human
50
diseases, including respiratory tract infections, traumatic skin and soft tissue infections,
51
bacteremia, and other infections involving almost all human organs [2,3,4]. Innate immunity
52
is a critical host defense system against mycobacterial infection that detects a variety of
53
mycobacterial-derived molecular patterns while inducing proinflammatory mediators and
54
antimicrobial proteins [5,6,7]. Numerous pattern-recognition receptors, such as Toll-like
55
receptors (TLRs), are involved in the recognition of mycobacterial products. These
56
mechanisms also trigger complex intracellular signaling activation, culminating in the
57
activation of nuclear factor (NF)-κB and mitogen-activated protein kinase (MAPK) signaling
58
in innate immune cells [8,9]. Activation of innate immune signaling leads to the production of
59
proinflammatory cytokines, including tumor necrosis factor TNF-α, interleukin (IL)-6, IL-1β,
60
and IL-12 [8,10].
TE D
M AN U
SC
RI PT
47
The development of molecular genetic approaches, such as whole-genome sequencing,
62
has markedly enhanced our understanding of various properties of Mab [11]. The
63
identification and immunological characterization of essential Mab genes contributes to the
64
development of novel protective and therapeutic strategies against Mab infection. However,
65
little is known about the function of many Mab genes in terms of their interactions with host
66
immune cells that elicit innate immune responses during Mab infection. In Mycobacterium
67
tuberculosis (Mtb), a widely characterized pathogen, five type VII secretion systems are
68
responsible for exporting proteins and members of the ESX family, which are involved in
69
tuberculosis pathogenesis and survival within host cells [12,13,14]. The early secreted
70
antigenic target of 6 kDa (ESAT-6)/culture filtrate protein of 10 kDa (CFP-10) complex,
71
secreted by the ESX-1 secretion system (also known as the RD1 region), plays an essential
AC C
EP
61
ACCEPTED MANUSCRIPT role in pathogenesis and immune activation during Mtb infection [15]. Furthermore, the ESX-
73
5 secretion system of pathogenic mycobacteria modulates the macrophage response in M.
74
marinum [16]. Compared to the ESX genomic location in Mtb, much less is known about the
75
immunological functions of the Mab ESX region. Mab only has two conserved ESX gene
76
clusters (ESX-3 and ESX-4) [17,18]. ESX-3 is conserved in all mycobacterial species [19]
77
and has a role in promoting mycobacterial virulence [20]. ESX-3 is also an essential
78
secretion system for iron and zinc homeostasis in M. tuberculosis and is consequently linked
79
to adaptations of M. tuberculosis in low zinc environments [21].Although this locus has been
80
implicated in mycobacterial growth [19], the function of ESX-3 has not been widely studied in
81
terms of host–pathogen interaction during Mab infection. Mab includes EsxG and EsxH
82
proteins, major proteins encoded by the esx-3 region, which show a high level of homology
83
with EsxG and EsxH from Mtb. The present study reports evidence showing an important
84
role for Mab ESX-3 in the induction of host immunopathological responses and increased
85
mycobacterial growth during infection.
89 90 91 92 93 94 95
SC
M AN U
TE D
88
EP
87
AC C
86
RI PT
72
ACCEPTED MANUSCRIPT 96
2. Material and Methods
97
2.1. Inactivation of esx gene cluster The mutation construct for the ESX-3 gene cluster was generated by PCR-
99
amplification from Mab ATCC 19977 genomic DNA as a template. The primer pair pJV531F
100
(CCCAAGCTTAGACCACTTCGCGGGCGACGG) and pJV531R (CTACCTGCAGCACTTAC
101
AGCCCTTCACCCG), including HindIII and PstI sites, respectively, was used to amplify
102
fragment 1, which consists of N-terminal amino acids together with a region ∼925 bp
103
downstream of Mab 2234c. Similarly, the primers pJV532F (CTACCTGCAGGTGCTGGG
104
GCGAGCACTTGC)
105
containing PstI and XbaI sites, respectively, were used for amplification of fragment 2 (1045
106
bp), which includes 140 bp of Mab 2224c. In more detail, fragment 1 was subcloned into
107
HindIII/PstI-digested pBluescript II SK(+) and fragment 2 was subsequently subcloned into
108
PstI/XbaI-digested pBluescript II SK(+) harboring fragment 1 to generate pBSK-∆esx. The
109
zeocin
110
(CTACCTGCAGCGCTAGCTCGAGCACGTGTTGACAATTAATCATCGGCATAGTATATC)
111
and ZeoR4pcD (CTAGCTGCAGATCTCGTAGCACGTGTCAGTC) from pcDNA3.1/Zeo(+). It
112
was digested with PstI, purified, and cloned into the PstI site of pBSK-∆esx to generate
113
pBSK-∆esx::zeo. Allelic-exchange substrate (AES) was amplified from pBSK-∆esx::zeo and
114
used to perform mutagenesis in Mab. The strain containing pJV53 was cultured and
115
incubated with 0.2% acetamide. Electrocompetent cells were prepared with ice-cold 10%
116
glycerol solution. The competent cells were electroporated with 100 ng of AES and plated on
117
50 µg/mL zeocin after 24 h of incubation at 37 °C. Muta tion events were verified by PCR and
118
sequencing.
(CGTCTAGAAGTGCCCTGCCCTCGCACGTC),
M AN U
was
pJV532R
amplified
using
two
different
primers,
Zeo-F2
AC C
EP
TE D
cassette
and
SC
RI PT
98
119 120
2.2. Bacteria culture condition, enumeration and In vitro growth kinetics
121 122
In vivo examinations were performed with Mab ATCC 19977; Wild-type (WT) and
ACCEPTED MANUSCRIPT 123
∆esx. Both strains were grown for 4 days, at 37°C, in M iddlebrook 7H9 broth supplemented
124
with albumin-dextrose-catalase (ADC, Difco) with daily agitation. These cultures were further
125
diluted serially (10-fold) to quantify colony-forming units (CFU)/mL.
126
spread on Middlebrook 7H10 agar media supplemented with 10% OADC (oleic acid, albumin,
127
dextrose and catalase, Difco) and incubated as described above until colonies were visible.
128
The visible Mab colonies were counted and adjusted based on the dilution factor. According
129
to this CFU determination, stocks of 1 × 108 CFU/mL were prepared and stored at -80°C until
130
used. Prior to infection, frozen stocks were thawed and 10-fold serial dilutions were prepared
131
in PBS plus 0.05% Tween-80 (PBST) before infection. To determine whether esx-3 gene
132
cluster disruption has brought in any change in the in vitro cultivation, we compared the
133
growth rates of Mab WT or ∆esx under enriched Middlebrook 7H9 broth supplemented with
134
10% ADC. A growth assay was performed in 3 mL shaking cultures at 37°C. The OD600 was
135
measured every 12 h for 4 days. All the experiments were performed in triplicate and
136
standard deviations were determined.
RI PT
M AN U
SC
2.3. Mice and cells
TE D
137 138
100 µL aliquots were
Wild-type female C57BL/6 mice (aged 6–8 weeks) were purchased from SAMTAKO
140
BIO (Gyeonggi-do, Korea) and were maintained under specific pathogen-free conditions. All
141
animal-related procedures were reviewed and approved by the Institutional Animal Care and
142
Use Committee, Chungnam National University School of Medicine (CNUH-014-A0008;
143
Daejeon, Korea). All animal procedures were conducted in accordance with guidelines of the
144
Korean Food and Drug Administration (KFDA). Murine bone marrow-derived macrophages
145
(BMDMs) were isolated and differentiated by growth for 4–5 days in medium containing
146
macrophage colony-stimulating factor (25 ng/mL; R&D Systems, 416-ML). The culture
147
medium was Dulbecco’s modified Eagle’s medium (DMEM; Lonza, 12-604F, NJ, USA),
148
which contained 10% FBS (Lonza, BW14-503E) and penicillin–streptomycin–amphotericin B
149
(Lonza, 17-745E). Human monocyte derived macrophages (MDMs) were prepared as
AC C
EP
139
ACCEPTED MANUSCRIPT 150
described previously [22]. Briefly, human monocytes were isolated from blood obtained from
151
healthy volunteers. The buffy coat was collected using a Ficoll gradient and monocytes were
152
enriched by adherence to tissue culture plastic. The Institutional Research and Ethics
153
Committee at Chungnam National University Hospital approved this study.
155
RI PT
154
2.4. Infection macrophages, mouse infection, histopathology, and bacterial counts
For infection, Mab WT and ∆esx were added to macrophages at 1:1 or 1:10
157
multiplicity of infection (MOI). After 4h of infection, extracellular mycobacteria were washed
158
out and infected macrophages were maintained in culture medium at 37°C and 5% CO 2 for 3
159
days. For bacterial burdens in the spleen and liver, mice per group were intravenously
160
infected with 1×107 CFU/mouse of Mab WT or ∆esx. Lungs, livers, and spleens were
161
harvested, and homogenates were counted at different times (1, 7, and 14 days) after
162
infection. For bacterial counting, the number of viable bacteria in each organ was determined
163
by plating serial dilutions of whole-organ homogenates on Middlebrook 7H10 agar
164
supplemented with OADC (Difco, Detroit, MI, USA). Colonies were counted after 3–5 days of
165
incubation at 37 °C, and the results were calculate d as the mean log10 CFU per organ.
166
Control mice were injected with PBST. For secretion of serum cytokine levels, 1×107 bacilli of
167
Mab WT or ∆esx were intravenously infected. ELISA was used to evaluate the levels of pro-
168
inflammatory cytokines, such as TNF-α and IL-6, in the infected lungs of mice within one day
169
post-infection. For IHC staining findings (for lung), groups of five mice each were
170
anaesthetized, their trachea exposed via a small midline incision. Each mice were infected
171
intratracheally with 5×105 CFU of Mab WT or ∆esx per mouse in 50 µL PBST. Lung samples
172
were fixed in 10% formalin and embedded in paraffin wax. Sections were then cut and
173
stained with hematoxylin and eosin. Inflammation in lung sections was graded for severity by
174
scanning multiple random fields in three sections of each tissue per mouse. An overall
175
histopathological score was assigned to each tissue in each animal based on the extent of
176
granulomatous inflammation as follows: 0 = no lesion, 1 = minimal lesion (1–10% of tissue in
AC C
EP
TE D
M AN U
SC
156
ACCEPTED MANUSCRIPT 177
section involved), 2 = mild lesion (11–30% involved), 3 = moderate lesion (30–50% involved),
178
4 = marked lesion (50–80% involved), and 5 = severe lesion (> 80% involved), as described
179
previously [20].
180
2.5. Reagents and antibodies Ultrapure lipopolysaccharide (LPS; tlrl-3pelps) was purchased from InvivoGen (San
182
Diego, USA). DAPI was purchased from Sigma. For western blotting, specific antibodies
183
(Abs) against phospho-SAPK/JNK (4668), phospho-p44/42 MAPK (ERK1/2) (9101), and
184
phospho-p38 MAP Kinase (9211) were obtained from Cell Signaling Technology (Beverly,
185
MA, USA). Anti-IκB-α (sc-371) and anti-actin (sc-1616) were obtained from Santa Cruz
186
Biotechnology (Santa Cruz, CA, USA). For IHC staining, paraffin wax-embedded lung
187
sections were stained using anti-COX2 (ab15191), anti-neutrophil (ab2557), and anti-iNOS
188
(ab3523) Abs biotin-conjugated rabbit anti-mouse IgG, as well as a peroxidase-conjugated
189
streptavidin Ab.
M AN U
SC
RI PT
181
190
2.6. RNA extraction, quantitative real-time PCR, enzyme-linked immunosorbent assays
192
(ELISA) and Western blotting
TE D
191
Total RNA was extracted from cells using the TRIzol reagent (Thermo Fisher
194
Scientific, 15596-026) according to the manufacturer’s protocol. Real-time PCR reactions
195
were performed according to the manufacturer’s instructions (SYBR green PCR master mix,
196
Qiagen), and thermal cycling was performed in a Rotor Gene 6000 instrument (Qiagen).
197
Primer sequences were as follows: mTNFα (forward: AGCACAGAAAGCATGAT
198
CCG, reverse: CTGATGAGAGGGAGGCCATT), mIL6 (forward: ACAAAGCCAGAGTCCTTC
199
AGA, reverse: TGGTCCTTAGCCACTCCTTC), mIL1β (forward: TGACGGACCCCAAAAGAT
200
GA, reverse: AAAGACACAGGTAGCTGCCA), mIL12p40 (forward: AGGTCACACTGGACCA
201
AAGG, reverse: TGGTTTGATGATGTCCCTGA), mβactin (forward: CCACCATGTACCCAGG
202
CATT, reverse: AGGGTGTAAAACGCAGCTCA), hTNFα (forward: GGCGTGGAGCTGAGAG
203
ATAAC, reverse: GGTGTGGGTGAGGAGCACAT), hIL6 (forward: TGTGAAAGCAGCAAAG
AC C
EP
193
ACCEPTED MANUSCRIPT AGGCACTG, reverse: ACAGCTCTGGCTTGTTCCTCACTA), and hβactin (forward: CACCAT
205
TGGCAATGAGCGGTTC, reverse: AGGTCTTTGCGGATGTCCACGT). In the sandwich
206
ELISA, serum and cell culture supernatants were analyzed using a Mouse BD OptEIA Set
207
ELISA Kit (BD Biosciences, USA) to detect TNF-α (558534), IL-6 (555240), IL-1β (559603),
208
and IL-12p40 (555165). The Human Ready-SET-Go ELISA kit (eBioscience, USA) was used
209
to detect TNF-α (88-7346) and IL-6 (88-7066). The limit of detection of the assay indicated
210
by the manufacturer (BD OptEIA Set ELISA Kit) was mouse 15 pg/ml (for mouse TNF-α), 4
211
pg/ml (for mouse IL-6, IL-1β, IL-12p40, and human TNF-α) and 2 pg/ml (for human IL-6). For
212
Western blotting, cell lysis was performed with RIPA buffer (50 mM Tris-HCl, pH 8.0, 150 mM
213
NaCl, 0.1% SDS, 1% NP-40, 0.5% deoxycholate and protease inhibitors) at 4 °C for 60 min.
214
The protein extracts were boiled in SDS sample buffer, loaded onto a 12% SDS-
215
polyacrylamide gel for electrophoresis, and transferred to a polyvinylidene difluoride
216
membrane (Millipore, IPVH00010). Signals were visualized with ECL solution (Millipore,
217
WBKL S0500) and detected with an UVitec Alliance mini-chemiluminescence device (UVitec,
218
Rugby, UK). The ImageJ software was used for densitometric analysis of the blots.
219
221
2.7. Immunofluorescence microscopy of NF-κB p65 translocation Translocation
of
NF-κBp65
EP
220
TE D
M AN U
SC
RI PT
204
into
the
nucleus
was
detected
using
immunofluorescence staining. Briefly, cells were infected with Mab WT or ∆esx for 30 min
223
and then fixed with 4% paraformaldehyde in PBS for 10 min. Cells were permeabilized with
224
0.25% Triton X-100 in PBS for 10 min and stained with anti-mouse NF-κB p65 (1:400, for 18
225
h at 4 °C; sc-372, Santa Cruz Biotechnology, Inc.) and anti-rabbit AlexaFluro 488 (1:400, for
226
2 h; A-11008, Invitrogen) at room temperature (RT). Nuclei were stained by incubation with
227
DAPI (Sigma) for 2 min. After mounting, fluorescence images were acquired using a
228
confocal laser-scanning microscope (LSM 710; Carl Zeiss, Jena, Germany).
AC C
222
229 230
2.8. NF-κB Luciferase reporter assays
ACCEPTED MANUSCRIPT Transduction with the NF-κB-Luciferase adenovirus (Genetransfer Vector Core;
232
Iowa City, IA, USA) was performed for 36 h, followed by infection with Mab WT or ∆esx for 6
233
h. Infected cells were washed three times in PBS, and cell extracts were prepared by adding
234
100 µL of 1× Passive Reporter Lysis Buffer (Promega, Madison, WI, USA). Luciferase
235
activity was measured using the Luciferase Assay System (Promega) according to the
236
manufacturer’s instructions.
RI PT
231
237
2.9. Recombinant protein purification
SC
238
The coding regions for EsxG (MAB_2229c) and EsxH (MAB_2228c) were subcloned
240
into NcoI and XhoI restriction sites of the pHis-parallel1 and pGST-parallel1 vectors,
241
respectively, containing recombinant TEV protease (rTEV) cleavage sites [24]. ClearColi
242
BL21 (DE3) cells (Lucigen, Middleton, USA) harboring each plasmid were grown in LB
243
medium containing ampicillin at 37 °C until they re ached an OD600 of 0.4–0.5. After cooling to
244
18 °C, protein expression was induced with 0.5 mM I PTG overnight. The cells expressing
245
each protein were then harvested and re-suspended in cooled buffer (50 mM Tris-HCl, pH
246
8.0, 300 mM NaCl, and 5% glycerol). The cell suspension was lysed with an ultra-high-
247
pressure homogenizer (UHPH; BEE International, USA). The expressed EsxG and EsxH
248
proteins were then purified by Ni-NTA agarose (Invitrogen, Carlsbad, CA) and GST agarose
249
(GE Healthcare, USA) affinity chromatography, respectively. GST-fused EsxH was further
250
purified by treatment with rTEV protease (Invitrogen) to remove GST and additional GST-
251
affinity chromatography. A complex of purified His-tagged EsxG and tag-free EsxH proteins
252
spontaneously formed upon mixing in a ratio of one to one. This complex was subjected to
253
size-exclusion chromatography for further purification. The complex protein was analyzed by
254
SDS-PAGE followed by Coomassie staining. Removal of endotoxin from recombinant
255
proteins was performed using polymyxin B-agarose (Sigma, USA) according to the
256
manufacturer’s protocol. Contamination with endotoxin was assessed with the Limulus
257
Amebocyte Lysate (LAL) QCL-1000 assay (Lonza, Walkersville, USA).
AC C
EP
TE D
M AN U
239
ACCEPTED MANUSCRIPT 258 259
2.10. Statistical Analyses All data obtained from independent experiments were analyzed by two-way analysis
261
of variance (ANOVA) with Bonferroni post-tests or one-way ANOVA with Bonferroni’s multiple
262
comparison test. Results are presented as the mean and standard error of the mean (SEM).
263
Differences were considered statistically significant when P < 0.05.
RI PT
260
264
3. Results
266
3.1. Construction of Mab mutants using a recombineering system
M AN U
SC
265
To study the functional role of ESX-3, recombineering was used to replace structural
268
gene regions with a zeocin cassette to provide resistance to zeocin [25]. Schematic
269
representations of the ESX-3 region genes in Mab WT and ∆esx mutant are shown in
270
Supplementary figure 1A and 1B, respectively. The resulting ∆esx strain was confirmed by
271
PCR using primers for the genomic region outside of the ESX-3 flanking regions. PCR
272
products (expected size 2.4 kb) would only be obtained if the zeocin cassette had been
273
inserted into the correct location on the chromosome. The expected PCR product size was
274
obtained from putative ∆esx; no product was obtained for WT Mab ATCC 19977 (13.7 kb;
275
Supplementary figure 1C). The amplicon was further analyzed by sequencing, which
276
confirmed the clear deletion of esx-3 regions from the genome (data not shown).
277
Furthermore, individual gene disruption was validated by PCR using individual gene-specific
278
primers (Supplementary figure 1D).
EP
AC C
279
TE D
267
280
3.2. Esx-3 locus is required for pathological changes during the acute phase of Mab infection
281
To determine whether esx-3 gene cluster disruption has brought in any change in the
282
in vitro cultivation, we compared the growth rates of Mab WT or ∆esx. Differences in growth
283
rate were compared using a nonparametric t test. As shown in Fig. 1A, the ∆esx did not
ACCEPTED MANUSCRIPT displayed a significantly reduced growth rate and doubling time compared to that of the Mab
285
WT. The mutant reached a stationary phase at 72 hours after inoculation with a similar
286
density compared to the WT (Fig. 1A, P=0.6270). Based on similarity of growth patterns
287
between Mab WT and ∆esx, we further assessed the role of esx-3 in Mab survival inside
288
macrophages. For this, survival of ∆esx was studied in BMDMs and compared with that of
289
Mab WT. The results showed that within 3 days, BMDMs were unable to eliminate the Mab
290
WT strain. As shown in Fig.1B, intracellular growth of Mab WT was significantly increased in
291
BMDMs compared with ∆esx at 3 days after infection. Similar findings were observed in data
292
from different MOIs (Fig.1B), suggesting that esx-3 is required for intracellular survival of
293
Mab. This finding was further studied using an in vivo acute model of infection. At days 7 and
294
14, the bacterial load in the spleen and liver was determined. As shown in Fig.1C,
295
significantly decreased splenic and hepatic bacillary loads were found in mice infected with
296
∆esx on day 7 after infection compared with those from mice infected with the WT strain. At
297
14 days post-infection, there were no change for bacterial growth in the livers of ∆esx
298
infected mice (Fig.1C). The results presented above show that growth of the ∆esx strain was
299
inhibited in mouse organs.
TE D
M AN U
SC
RI PT
284
To this end, we investigated whether mice infected with ∆esx and Mab WT strains
301
show different pathological responses. As shown in Fig.1D, the lungs of mice infected with
302
Mab WT exhibited extensive pathological changes at 7 days post-infection. In more detail,
303
the lung sections of mice infected with Mab WT exhibited severe lung pathology
304
characterized by much more dense alveolar spaces and increased granulomatous infiltrate.
305
However, significantly less granulomatous infiltrate was observed in ∆esx-infected animals.
306
Quantitative scoring of histopathological changes confirmed that the Mab WT group (n=5)
307
showed much more severe lung pathology than the ∆esx group at 7 days post-infection
308
(Fig.1D). Together, these pathological changes demonstrate that esx-3 influences the
309
pathogenesis of Mab in mice.
310
AC C
EP
300
ACCEPTED MANUSCRIPT 311
3.3. Mab ∆esx infection induces less inflammatory and pathological responses in vivo Mab vigorously activates innate immune responses in macrophages through
313
interactions between TLR2 and dectin-1 [26]. However, the role of the Mab esx-3 locus is not
314
well known in mice or macrophages. The serum levels of TNF-α and IL-6 in C57BL/6 mice
315
after infection were analyzed to examine if mice infected with ∆esx produced a more
316
attenuated inflammatory response than those infected with Mab WT. As shown in Fig.2A,
317
∆esx elicited a reduced amount of both TNF-α and IL-6 compared to the WT strain,
318
especially at one day post-infection.
SC
RI PT
312
319
Expression of cyclooxygenase 2 (COX2), inducible nitric oxide synthase (iNOS), and
321
neutrophils in lungs was further evaluated by immunohistochemistry. Immunoreactivity
322
against three antibodies (COX-2, iNOS, and neutrophil) was investigated in lung tissues
323
infected with Mab WT or ∆esx strains (Fig.2B and 2C). The amount of positively stained cells
324
was evaluated to calculate the percent of positive cells for scoring. As shown in Fig.2B,
325
COX-2, iNOS, and neutrophil staining in lung sections differed significantly between the
326
infected strains. Mab WT infected lung tissue samples showed >58% COX-2 and >79%
327
iNOS positive expression rates in immunohistochemical scoring (Fig.2C). In contrast, ∆esx
328
infected lung tissues showed lower positive rates for COX-2 (25%) and iNOS (52%)
329
expression. In addition, ∆esx infected lung tissues had lower rates of neutrophil infiltration
330
compared to those infected with Mab WT (Fig.2B and 2C). Together, these data suggest that
331
systemic and local inflammatory responses are markedly reduced in ∆esx-infected mice
332
compared with those of Mab WT-infected mice.
TE D
EP
AC C
333
M AN U
320
334
3.4. Mab ∆esx leads to less proinflammatory cytokine production in murine and human
335
macrophages compared to WT strain
336
The contribution of the ESX-3 region to pro-inflammatory responses was further
337
examined in murine and human macrophages. Proinflammatory cytokine generation was
ACCEPTED MANUSCRIPT compared for Mab WT- and ∆esx-infected BMDMs as well as human monocyte-derived
339
macrophages (MDMs). Mab WT robustly induced mRNA expression of proinflammatory
340
cytokines (TNF-α, IL-6, IL-1β, and IL-12 p40) from BMDMs after 3 h of infection. The mRNA
341
levels of proinflammatory cytokines induced by ∆esx were significantly lower than those
342
induced by Mab WT at different time points, as shown in Fig.3A. BMDMs infected with ∆esx
343
also produced smaller amounts of proinflammatory cytokines after 18 or 48 h of infection
344
compared to those infected with the Mab WT strain (Fig.3B).
SC
345
RI PT
338
The mRNA and protein expression of proinflammatory cytokines in human MDMs was
347
further examined after Mab WT or ∆esx infection. Similar to findings observed in murine
348
BMDMs, human MDMs tend to produce less TNF-α and IL-6 mRNA at different time points
349
(3 and 6 h for TNF-α; 6 and 18 h for IL-6; Fig.3C) in response to ∆esx than in response to
350
the WT strain. In addition, ∆esx infection produced smaller amounts of TNF-α and IL-6 in
351
MDMs at different time points (from 6 to 18 h for TNF-α; from 6 to 48 h for IL-6) compared to
352
Mab WT infection (Fig.3D). These results demonstrate that the ESX-3 region of Mab plays a
353
role in the induction of inflammatory responses in murine and human macrophages.
TE D
355
3.5. Mab ∆esx significantly attenuates activation of MAPK signaling in macrophages
EP
354
M AN U
346
The MAPK pathways play a key role in the host inflammatory response during
357
mycobacterial infection [27,28]. To examine the molecular mechanisms underlying ESX-3-
358
mediated inflammatory responses, the activation of ERK, p38, and JNK MAPKs in BMDMs
359
infected with either Mab WT or ∆esx was examined. As shown in Fig.4A, Mab WT robustly
360
activated three families of MAPKs in BMDMs after infection in a time-dependent manner. As
361
expected, the ∆esx-infected BMDMs showed less phosphorylation of ERK, p38, and JNK
362
MAPKs at different time points compared to WT-infected BMDMs (Fig.4A). Densitometric
363
analysis showed that the phosphorylation levels of ERK, p38, and JNK MAPKs were
364
significantly decreased in BMDMs infected with ∆esx at 15 to 60 mins post-infection
AC C
356
ACCEPTED MANUSCRIPT 365
compared to those infected with the WT strain (Fig.4B). Moreover, the ∆esx-induced
366
phosphorylation of ERK, p38, and JNK MAPKs was significantly decreased in BMDMs
367
compared with those infected by WT (Fig.4C). Taken together, these results suggest that the
368
ESX-3 region is associated with MAPK activation in BMDMs after infection.
RI PT
369 370
3.6. ESX-3 locus contributes to the activation of NF-κB signaling in macrophages during Mab
371
infection
We next examined whether the ESX-3 locus was involved in nuclear translocation and
373
activation of NF-κB, an essential transcriptional factor in inflammatory signaling [29], after
374
infection with ∆esx. Subcellular localization of NF-κB p65 in the nucleus was significantly
375
reduced in BMDMs infected with ∆esx compared to those infected with WT, as determined
376
by confocal microscopy after 30 min of infection (Fig.5A). This observation was further
377
analyzed by quantifying the effects of Mab WT and ∆esx on translocation of NF-κB/p65.
378
Quantification of cells from different fields showed a significantly lower percentage of NF-
379
κB/p65 translocation into nuclei in BMDMs infected with ∆esx compared with Mab WT
380
infection. Moreover, this relationship operated in a MOI-dependent manner (Fig.5B).
TE D
M AN U
SC
372
381
A NF-κB luciferase assay was also performed in BMDMs transduced with adenovirus
383
encoding a luciferase reporter plasmid containing response elements for NF-κB (Ad-NF-κB-
384
Luc). The activity of the NF-κB reporter gene was considerably reduced in BMDMs
385
transduced with Ad-NF-κB-Luc with ∆esx infection compared to those infected by Mab WT
386
(Fig.5C). As shown in Fig.5D, the effect of ∆esx on IκB-α degradation in BMDMs was also
387
examined. Degradation of IκB-α was prominent in BMDMs after 15-30 min of Mab WT
388
infection. However, few changes in IκB-α degradation were found in BMDMs after ∆esx
389
infection. Thus, the ESX-3 region enhanced activation of NF-κB signaling in BMDMs during
390
Mab infection.
391
AC C
EP
382
ACCEPTED MANUSCRIPT 392
3.7. rEsxGH protein is required for synergistic synthesis of TNF-α and IL-6 in BMDMs
393
infected with Mab ∆esx Previous studies have shown multiple sequence alignments highlighting the conservation
395
of amino acids in EsxG and EsxH orthologs from several mycobacterial strains, but not from
396
Mab [13]. We re-performed multiple sequence alignments of the conserved amino acids in
397
EsxG (MAB 2229c, upper) and EsxH (MAB 2228c, lower) orthologs from Mab, Mtb H37Rv,
398
Mtb H37Ra, M. bovis, M. ulcerans, M. leprae, M. smegmatis, and M. marinum (Fig.6A).
399
Overall, the amino acid sequences of orthologs were well conserved.
SC
RI PT
394
400
To evaluate the immunological relevance of both proteins, recombinant EsxGH (rEsxGH)
402
complex was purified. A previous study showed that the Mtb proteins CFP‐10 (Rv0287) and
403
ESAT‐6 (Rv0288), homologue proteins of EsxG and EsxH, respectively, form tight
404
heterodimeric complexes in the solution [30]. Consistent with the previous result, size-
405
exclusion chromatography analysis revealed that EsxG and EsxH proteins were co-eluted at
406
a fraction corresponding to the EsxGH complex with a molecular weight of ~20 kDa (Fig.6B).
407
The complex was confirmed by SDS-PAGE analysis (Fig.6C).
TE D
408
M AN U
401
Subsequently, BMDMs were stimulated in vitro with purified rEsxGH and then subjected
410
to endotoxin removal using polymyxin B-agarose. The cellular responses were analyzed and
411
compared with the response to Mab WT and ∆esx. As seen in Fig.6D, treatment of BMDMs
412
with rEsxGH protein alone did not induce the release of TNF-α or IL-6. Proinflammatory
413
cytokines were induced at a very low level of TNF-α and IL-6 from BMDMs infected with
414
∆esx, as seen in Fig.3. Interestingly, the production of TNF-α and IL-6 was synergistically
415
increased in ∆esx-infected BMDM when combined with rEsxGH protein in a dose-dependent
416
manner. These data suggest that rEsxGH from the ESX-3 region can rescue the function of
417
the ESX-3 region through in vitro complementation. Together, the EsxG and EsxH proteins
418
of the Mab ESX-3 region are associated with host inflammatory responses during the course
AC C
EP
409
ACCEPTED MANUSCRIPT 419
of Mab infection.
420 421 422
4. Discussion In this study, we characterized the innate immune function of the Mab ESX-3 region by
424
constructing an ESX-3 (MAB 2224c-2234c)-deletional mutant strain of Mab (∆esx) in murine
425
bone marrow-derived macrophages (BMDMs) and in vivo. Compared to Mab wild type (Mab
426
ATCC 19977), ∆esx infection resulted in induction of less histopathology and inflammatory
427
mediator production in vivo. It also resulted in lower levels of inflammatory signaling and
428
cytokine production in macrophages. Additionally, intracellular bacterial survival was
429
significantly attenuated in ∆esx-infected conditions. In vitro complementation with
430
recombinant EsxG▪EsxH (rEsxGH) proteins, two major proteins encoded by the ESX-3
431
region in Mab [13], was also performed. This showed that restoration of inflammatory
432
cytokine production was as likely as with the wild-type strain. The present study reports
433
evidence showing an important role for Mab ESX-3 in the induction of host
434
immunopathological responses and increased mycobacterial growth during infection.
SC
M AN U
TE D
435
RI PT
423
Mab is one of the most frequent causes of lung disease, accounting for around 80% of
437
pulmonary infections caused by rapidly growing mycobacteria [3]. One of the most serious
438
clinical burdens in an emerging Mab infection is chemotherapy difficulties, due to the intrinsic
439
drug resistance of Mab to various antibiotics [31]. There is an urgent need for the
440
development of new vaccines and therapeutic strategies to control Mab infection in both
441
immunocompetent and immunocompromized patients [32,33]. To this end, a more
442
comprehensive understanding of the host–pathogen interaction should be preceded by the
443
identification and functional characterization of essential Mab genes. Our findings identify the
444
Mab ESX-3 region as important for intracellular bacterial survival and elicitation of excessive
445
inflammatory and pathological responses during Mab infection.
AC C
EP
436
ACCEPTED MANUSCRIPT 446
In more detail, deletion of the Mab ESX-3 region leads to attenuated growth and
448
persistence in both macrophages. In addition, ∆esx infected organs such as spleen and liver
449
rapidly underwent a progressive reduction of CFU in comparison with wild-type strain at 7
450
days after infection. Mycobacterial virulence can be measured by the ability of bacteria to
451
invade, grow, and persist not only in macrophages, but also in an in vivo rodent model.
452
Sweeney et al. previously showed that the IKE (Mycobacterium smegmatis strain with
453
deletion of the esx-3 region) strain could not elicit different IL-6 amounts with parental and
454
∆esx-1 Msmeg. Fredric et al. also reported that Esx-1 deficient (∆RD1) M. marinum
455
appeared to perturb the host immune response [34]. In more detail, ∆RD1 M. marinum alters
456
the immune response by decreasing TNFα and IL-6 production. The presence of Esx-1
457
promotes NFκB activation in macrophages in vitro, which could account for increased TNFα
458
and IL-6 seen with infections by WT M. marinum in vivo. In this study, we observed innate
459
immune responses that were similar to those seen in the host immune response of ∆RD1 M.
460
marinum. This is because the Mab ESX-3 cluster harbors esxG (Rv0287, ESAT-6 like
461
protein), which has high homology with M. marinum esxG (MMAR 0546; ESAT-6 like protein)
462
(74% identities and 80% positives). The generation of proinflammatory cytokines (TNF-α, IL-
463
6, IL-1β, and IL-12p40) is significantly decreased by the ∆esx strain in macrophages from
464
mice and humans. This is the first report that Mab ESX-3 is involved in exacerbated
465
inflammatory responses, as well as disease pathology and reduced bacillary control, during
466
infection. TNF-α is a key proinflammatory cytokine that mediates mycobacterial killing, host
467
defense, chemokine expression, and granuloma formation [35,36]. However, excessive
468
levels of TNF-α can lead to detrimental effects in the host. For example, excessive secretion
469
of TNF-α has been implicated in clinical worsening and tissue damage, whereas TNF-α
470
reduction has been correlated with decreased granuloma size and necrosis [37]. Thus, the
471
appropriate induction and control of this cytokine are thought to be key in host-directed
472
responses against tuberculosis [38]. Our report suggests that the Mab esx-3 region is
AC C
EP
TE D
M AN U
SC
RI PT
447
ACCEPTED MANUSCRIPT 473
involved in serum cytokine production that subsequently influences virulence in a mouse
474
model of infection.
475
Inflammatory responses triggered by mycobacterial infection lead to the robust
477
activation of intracellular signaling cascades involving three subfamilies of MAPKs and NF-
478
κB activation [8,26]. We also found that macrophage inflammatory signaling (NF-κB and
479
MAPK) is markedly downregulated by ∆esx infection. Indeed, there have been many reports
480
of in vitro and in vivo immune-modulating activity of the ESAT-6 antigen of Mtb. The ESAT-6
481
antigen elicited vaccine-enhancing Th17 immune responses through TLR2/MyD88 signaling
482
[39]. In contrast, RD-1 region antigens played the key role of down-regulating the functions
483
of macrophages, potentially contributing to Mtb virulence [40]. Previous studies also showed
484
that disruption of the M. marinum PPE38 gene resulted in reduced levels of TNF-α and IL-6
485
secretion in infected macrophages [41]. BLAST analysis revealed that MAB_2230c within
486
the ESX-3 gene cluster shares intermediate homology (~35%) with M. marinum PPE38
487
(data not shown). Taken together, our data suggest that the ESX-3 region may contribute to
488
excessive inflammatory responses and signaling activation in host macrophages.
SC
M AN U
TE D
489
RI PT
476
Efficiently mounting host defenses against mycobacterial infection depends on both
491
restriction of bacterial replication and prevention of overwhelming inflammatory responses
492
[42]. The immunopathological responses to Mab are poorly characterized compared to the
493
widely studied Mtb infection. The name “Mab” originated from abscess formation during
494
infection [43]. Clinical manifestations of Mab infection are often related to abscess
495
formations that require surgical treatment and severe inflammatory responses, such as
496
ulcerative, abscess-forming lesions [44,45]. In this study, we report that Mab infection
497
resulted in markedly increased granulomatous infiltrate and inflammatory infiltrates in mouse
498
lungs. We also found that the infiltration of neutrophils and immune cells expressing COX-2
499
and iNOS was markedly increased in mouse tissues within 1 week of infection with the Mab
AC C
EP
490
ACCEPTED MANUSCRIPT WT strain. Notably, pathological responses found in Mab WT-infected lungs and other
501
tissues were significantly attenuated compared to those from ∆esx-infected mice. These
502
data indicate that the Mab ESX-3 region is important in Mab pathogenesis and virulence
503
during infection.
RI PT
500
504
In this study, we were unable to complement the Mab WT strain with a mutant strain
506
given the current genetic tools. As with the M. smegmatis IKE strain, we could not
507
complement with cosmid pYUB1336, which harbors an intact M. tuberculosis ESX-3 locus
508
(Rv0282–Rv0292) [20]. We speculate that we would have been unable to complement Esx-3
509
function in an M. smegmatis mutant even if it were expressed pYUB1336 in this species,
510
suggesting that esx-3 functions are species-specific. Other E. coli/ Mycobacterial expression
511
vectors using the hsp60 promoter fused with the ESX-3 region (MAB 2224c-2234c) were
512
also unable to complement, probably due to overexpression of a gene cluster with several
513
membrane proteins. To compensate for this in an alternative way, recombinant proteins
514
rEsxG and rEsxH were generated from esxH and esxH genes, which were expected to be
515
the main functional genes in the Mab ESX-3 region. The ∆esx phenotype was partly rescued
516
when ∆esx was co-incubated with rEsxG and rEsxH. Although the recombinant protein alone
517
was unable to induce proinflammatory cytokine release, ∆esx - rEsxG and rEsxH could elicit
518
a dose-dependent increase in TNF-α and IL-6 levels in macrophages to levels observed in
519
Mab WT strain-infected cells. Recent studies showed that Mtb type VII effector EsxH, in
520
complex with EsxG, is involved in impaired phagosomal maturation by disrupting the
521
endosomal sorting complex required for transport (ESCRT) function, restricting intracellular
522
bacterial growth [46]. Combined with our data, this suggests that at least two proteins, esxG
523
and esxH gene products, may contribute to the pathological responses induced by the Mab
524
ESX-3 region. Further studies are needed to clarify the distinct function of each gene located
525
within the ESX-3 region of the Mab genome.
AC C
EP
TE D
M AN U
SC
505
ACCEPTED MANUSCRIPT 526
In summary, we report a function of the Mab ESX-3 cluster with regard to virulence and
528
replication failure in a mouse model of infection. The absence of Mab ∆esx resulted in less
529
accumulation of neutrophils and inflammatory mediator release in vivo. Furthermore, Mab
530
ESX-3 plays an important role in excessive proinflammatory cytokine production through
531
modulation of MAPKs and NF-κB in macrophages. The EsxGH proteins of the Mab ESX-3
532
region contributed to a rescue of the attenuated inflammatory responses induced by the
533
∆esx strain. The immunopathological action of the Mab ESX-3 region may be associated
534
with Mab virulence and inflammatory responses during the course of Mab infection.
SC
RI PT
527
536
M AN U
535
Acknowledgements
We thank D. M. Shin and J. J. Kim for helpful discussion and reagents. We thank D.
538
Ray for critical reading of the manuscript. This work was supported by a grant of the Korea
539
Health Technology R&D Project through the Korea Health Industry Development Institute
540
(KHIDI), by the National Research Foundation of Korea (NRF) grant funded by the Korean
541
government (MSIP) (2011-0030049) at Hanyang University, and by the Basic Science
542
Research Program through the NRF funded by the Ministry of Education (NRF-
543
2014R1A6A1029617) .
545 546 547 548 549 550
EP
AC C
544
TE D
537
Conflict of interest
No conflict of interest
ACCEPTED MANUSCRIPT References
552
[1] Field SK, Cowie RL. Lung disease due to the more common nontuberculous
553
mycobacteria. Chest 2006; 129:1653-72.
554
[2] Brown-Elliott BA, Wallace RJ Jr. Clinical and taxonomic status of pathogenic
555
nonpigmented or late-pigmenting rapidly growing mycobacteria. Clin Microbiol Rev
556
2002;15:716-46.
557
[3] Griffith DE, Aksamit T, Brown-Elliott BA, Catanzaro A, Daley C, Gordin F, et al. An official
558
ATS/IDSA statement: diagnosis, treatment, and prevention of nontuberculous mycobacterial
559
diseases. Am J Respir Crit Care Med 2007;175:367-416.
560
[4] Nessar R, Cambau E, Reyrat JM, Murray A, Gicquel B. Mycobacterium abscessus: a new
561
antibiotic nightmare. J Antimicrob Chemother 2012;67:810-8.
562
[5] Thoma-Uszynski S, Stenger S, Takeuchi O, Ochoa MT, Engele M, Sieling PA, et al.
563
Induction of direct antimicrobial activity through mammalian toll-like receptors. Science
564
2001;291:1544-7.
565
[6] Yamashiro LH, Oliveira SC, Báfica A. Innate immune sensing of nucleic acids from
566
mycobacteria. Microbes Infect 2014;16:991-7.
567
[7] Stamm CE, Collins AC, Shiloh MU. Sensing of Mycobacterium tuberculosis and
568
consequences to both host and bacillus. Immunol Rev 2015;264:204-19.
569
[8] Basu J, Shin DM, Jo EK. Mycobacterial signaling through toll-like receptors. Front Cell
570
Infect Microbiol 2012;2:145.
571
[9] Killick KE, Ní Cheallaigh C, O'Farrelly C, Hokamp K, MacHugh DE, Harris J. Receptor-
572
mediated recognition of mycobacterial pathogens. Cell Microbiol 2013;15:1484-95.
573
[10] Hossain MM, Norazmi MN. Pattern recognition receptors and cytokines in
574
Mycobacterium
575
2013;2013:179174.
576
[11] Howard ST. Recent progress towards understanding genetic variation in the
577
Mycobacterium abscessus complex. Tuberculosis (Edinb) 2013;93:S15-20.
AC C
EP
TE D
M AN U
SC
RI PT
551
tuberculosis
infection--the
double-edged
sword?
Biomed
Res
Int
ACCEPTED MANUSCRIPT [12] Stanley SA, Raghavan S, Hwang WW, Cox JS. Acute infection and macrophage
579
subversion by Mycobacterium tuberculosis require a specialized secretion system. Proc Natl
580
Acad Sci USA 2003;100:13001-6.
581
[13] Ilghari D, Lightbody KL, Veverka V, Waters LC, Muskett FW, Renshaw PS, et al.
582
Solution structure of the Mycobacterium tuberculosis EsxG.EsxH complex: functional
583
implications and comparisons with other M. tuberculosis Esx family complexes. J Biol Chem
584
2011;286:29993-30002.
585
[14] Liu W, Peng Y, Yin Y, Zhou Z, Zhou W, Dai Y. The involvement of NADPH oxidase-
586
mediated ROS in cytokine secretion from macrophages induced by Mycobacterium
587
tuberculosis ESAT-6. Inflammation 2014;37:880-92.
588
[15] Lewis KN, Liao R, Guinn KM, Hickey MJ, Smith S, Behr MA, et al. Deletion of RD1 from
589
Mycobacterium tuberculosis mimics bacille Calmette-Guérin attenuation. J Infect Dis
590
2003;187:117-23.
591
[16] Abdallah AM, Savage ND, van Zon M, Wilson L, Vandenbroucke-Grauls CM, van der
592
Wel NN, et al. The ESX-5 secretion system of Mycobacterium marinum modulates the
593
macrophage response. J Immunol 2008;181:7166-75.
594
[17] Choo SW, Wee WY, Ngeow YF, Mitchell W, Tan JL, Wong GJ, et al. Genomic
595
reconnaissance of clinical isolates of emerging human pathogen Mycobacterium abscessus
596
reveals high evolutionary potential. Sci Rep 2014;4:4061.
597
[18] Sassi M, Drancourt M. Genome analysis reveals three genomospecies in
598
Mycobacterium abscessus. BMC Genomics. 2014;15:359.
599
[19] Siegrist MS, Unnikrishnan M, McConnell MJ, Borowsky M, Cheng TY, Siddiqi N, et al.
600
Mycobacterial Esx-3 is required for mycobactin-mediated iron acquisition. Proc Natl Acad Sci
601
USA 2009;106:18792-7.
602
[20] Sweeney KA, Dao DN, Goldberg MF, Hsu T, Venkataswamy MM, Henao-Tamayo M, et
603
al. A recombinant Mycobacterium smegmatis induces potent bactericidal immunity against
604
Mycobacterium tuberculosis. Nat Med 2011;17:1261-8.
AC C
EP
TE D
M AN U
SC
RI PT
578
ACCEPTED MANUSCRIPT [21] Serafini A, Pisu D, Palù G, Rodriguez GM, Manganelli R. The ESX-3 secretion system is
606
necessary for iron and zinc homeostasis in Mycobacterium tuberculosis. PLoS One.
607
2013;8:e78351.
608
[22] Yang CS, Shin DM, Kim KH, Lee ZW, Lee CH, Park SG, et al. NADPH oxidase 2
609
interaction with TLR2 is required for efficient innate immune responses to mycobacteria via
610
cathelicidin expression. J Immunol 2009;182:3696-705.
611
[23] Wang J, Li BX, Ge PP, Li J, Wang Q, Gao GF, Qiu XB, Liu CH. Mycobacterium
612
tuberculosis suppresses innate immunity by coopting the host ubiquitin system. Nat Immunol.
613
2015;16:237-45.
614
[24] Sheffield P, Garrard S, Derewenda Z. Overcoming expression and purification problems
615
of RhoGDI using a family of "parallel" expression vectors. Protein Expr Purif 1999;15:34-9.
616
[25] van Kessel JC, Marinelli LJ, Hatfull GF. Recombineering mycobacteria and their phages.
617
Nat Rev Microbiol 2008;6:851-7.
618
[26] Shin DM, Yang CS, Yuk JM, Lee JY, Kim KH, Shin SJ, et al. Mycobacterium abscessus
619
activates the macrophage innate immune response via a physical and functional interaction
620
between TLR2 and dectin-1. Cell Microbiol 2008;10:1608-21.
621
[27] Zhou B, He Y, Zhang X, Xu J, Luo Y, Wang Y, et al. Targeting mycobacterium protein
622
tyrosine phosphatase B for antituberculosis agents. Proc Natl Acad Sci USA 2010;107:4573-
623
8.
624
[28] Seto S, Tsujimura K, Koide Y. Coronin-1a inhibits autophagosome formation around
625
Mycobacterium tuberculosis-containing phagosomes and assists mycobacterial survival in
626
macrophages. Cell Microbiol 2012;14:710-27.
627
[29] Kim TS1, Kim YS, Yoo H, Park YK, Jo EK. Mycobacterium massiliense induces
628
inflammatory responses in macrophages through Toll-like receptor 2 and c-Jun N-terminal
629
kinase. J Clin Immunol 2014;34:212-23.
630
[30] Renshaw PS, Lightbody KL, Veverka V, Muskett FW, Kelly G, Frenkiel TA, et al.
631
Structure and function of the complex formed by the tuberculosis virulence factors CFP-10
AC C
EP
TE D
M AN U
SC
RI PT
605
ACCEPTED MANUSCRIPT and ESAT-6. EMBO J 2005;24:2491-8.
633
[31] Lee MR, Sheng WH, Hung CC, Yu CJ, Lee LN, Hsueh PR. Mycobacterium abscessus
634
complex infections in humans. Emerg Infect Dis 2015;21:1638-46.
635
[32] Oh CT, Moon C, Park OK, Kwon SH, Jang J. Novel drug combination for
636
Mycobacterium abscessus disease therapy identified in a Drosophila infection model. J
637
Antimicrob Chemother 2014;69:1599-1607.
638
[33] Abdalla MY, Switzer BL, Goss CH, Aitken ML, Singh PK, Britigan BE. Gallium
639
compounds exhibit potential as new therapeutic agents against Mycobacterium abscessus.
640
Antimicrob Agents Chemother 2015;59: 4826-34.
641
[34] Carlsson F, Kim J, Dumitru C, Barck KH, Carano RA, Sun M, et al. Host-detrimental role
642
of Esx-1-mediated inflammasome activation in mycobacterial infection. PLoS Pathog.
643
2010;6:e1000895.
644
[35] Bermudez LE, Young LS. Tumor necrosis factor, alone or in combination with IL-2, but
645
not IFN-gamma, is associated with macrophage killing of Mycobacterium avium complex. J
646
Immunol 1988;140:3006-13.
647
[36] Flynn JL, Goldstein MM, Chan J, Triebold KJ, Pfeffer K, Lowenstein CJ, et al. Tumor
648
necrosis factor-alpha is required in the protective immune response against Mycobacterium
649
tuberculosis in mice. Immunity 1995;2:561-72.
650
[37] Bekker LG, Moreira AL, Bergtold A, Freeman S, Ryffel B, Kaplan G. Immunopathologic
651
effects of tumor necrosis factor alpha in murine mycobacterial infection are dose dependent.
652
Infect Immun 2000;68:6954-61.
653
[38] Dorhoi A, Kaufmann SH. Tumor necrosis factor alpha in mycobacterial infection. Semin
654
Immunol 2014;26:203-209.
655
[39] Chatterjee S, Dwivedi VP, Singh Y, Siddiqui I, Sharma P, Van Kaer L, et al. Early
656
secreted antigen ESAT-6 of Mycobacterium tuberculosis promotes protective T helper 17
657
cell responses in a toll-like receptor-2-dependent manner. PLoS Pathog 2011;7:e1002378.
658
[40] Pathak SK, Basu S, Basu KK, Banerjee A, Pathak S, Bhattacharyya A, et al. Direct
AC C
EP
TE D
M AN U
SC
RI PT
632
ACCEPTED MANUSCRIPT extracellular interaction between the early secreted antigen ESAT-6 of Mycobacterium
660
tuberculosis and TLR2 inhibits TLR signaling in macrophages. Nat Immunol 2007;8:610-8.
661
[41] Dong D, Wang D, Li M, Wang H, Yu J, Wang C, et al. PPE38 modulates the innate
662
immune response and is required for Mycobacterium marinum virulence. Infect Immun
663
2012;80:43-54.
664
[42] Nandi B, Behar SM. Regulation of neutrophils by interferon-γ limits lung inflammation
665
during tuberculosis infection. J Exp Med. 2011;208:2251-62.
666
[43] Moore M, Frerichs JB. An unusual acid-fast infection of the knee with subcutaneous,
667
abscess-like lesions of the gluteal region; report of a case with a study of the organism,
668
Mycobacterium abscessus, n. sp. J Invest Dermatol 1953;20:133-169.
669
[44] Song JY, Sohn JW, Jeong HW, Cheong HJ, Kim WJ, Kim MJ. An outbreak of post-
670
acupuncture cutaneous infection due to Mycobacterium abscessus. BMC Infect Dis 2006;6:6.
671
[45] Johnson MM, Odell JA. Nontuberculous mycobacterial pulmonary infections. J Thorac
672
Dis 2014;6:210-20.
673
[46] Mehra A, Zahra A, Thompson V, Sirisaengtaksin N, Wells A, Porto M, et al.
674
Mycobacterium tuberculosis type VII secreted effector EsxH targets host ESCRT to impair
675
trafficking. PLoS Pathog 2013;9:e100373.
676
.
679 680 681 682 683 684 685
SC
M AN U
TE D
EP
678
AC C
677
RI PT
659
ACCEPTED MANUSCRIPT 686
Figure legends
687
Fig.1. Mab esx-3 gene cluster is required for in vitro and in vivo growth.
689
A. Mab WT and ∆esx were grown in enriched Middlebrook 7H9 broth supplemented with
690
0.05% Tween and ADC and OD value was taken every 12 h at 600 nm. All data was
691
repeated in triplicates.
692
B. BMDMs were infected with different MOI (MOI of 1 or 10) of both either Mab WT or ∆esx,
693
washed, and macrophage lysates plated for CFU counts on 7H10 agar.
694
C. C57BL/6 mice were intravenously infected with 1×107 CFU of Mab WT and ∆esx strains.
695
Bacillary loads were determined in spleens and livers of C57BL/6 (n = 5) infected with Mab
696
WT and ∆esx at 1, 7, and 14 days post-infection. All data points are represented by log10
697
CFU values, and bars indicate standard errors.
698
D. Comparison of histopathological findings from C57BL/6 mice were intratracheally infected
699
with 5×105 CFU of Mab WT and ∆esx strains or PBST mock control. The figure depicts a
700
representative photograph of the extent of pathological damage of mice infected with PBST
701
mock control (n = 3), Mab WT (n = 5), and ∆esx (n = 5) at 7 days post-infection. Quantitative
702
scoring of histopathology is shown in the left lower panel. Data are presented as the mean ±
703
SEM of four independent experiments. *P < 0.05, **P <0.01, ***P < 0.001. Scale bars, 100
704
µm.
SC
M AN U
TE D
EP
AC C
705
RI PT
688
706
Fig.2. Esx-3 disruption induces less pro-inflammatory responses in vivo.
707
A. Blood serum levels of pro-inflammatory cytokines such as TNF-α (left) and IL-6 (right)
708
were measured by ELISA analysis from C57BL/6 mice were intravenously infected with
709
1×107 CFU of Mab WT and ∆esx strains (n = 9).
710
B. Expression of COX-2 and iNOS, as well as neutrophil infiltration in lung tissues from
711
C57BL/6 mice were intratracheally infected with 5×105 CFU of Mab WT (n = 5) and ∆esx
712
strains (n = 5) or PBST mock control (n = 3) at 7 days post-infection. Representative results
ACCEPTED MANUSCRIPT of immunohistochemistric analysis of expression of COX-2 and iNOS, and neutrophil
714
infiltration in lung tissues from mice infected with Mab WT or ∆esx (left). A brown color
715
indicates positive staining for the indicted proteins. Scale bars, 100 µm (for COX2 and iNOS)
716
or 50 µm (for Neutrophil).
717
C. Quantitative scoring of histopathologic findings (for B) by percentage of positively strained
718
cells. *P < 0.05, **P <0.01, ***P < 0.001.
719
RI PT
713
Fig.3. Proinflammatory cytokine generation in murine and human macrophages after
721
infection with Mab WT or ∆esx strain.
722
A and B. BMDMs were infected with Mab WT or ∆esx (MOI = 5) for the indicated times. The
723
mRNAs and supernatants were collected and subjected to qRT-PCR (for A) or ELISA
724
analysis (for B) to measure mRNA and protein expression of TNF-α, IL-6, IL-1β, and IL-
725
12p40.
726
C and D. Human MDMs were infected with Mab WT or ∆esx (MOI = 5) for the indicated
727
times. The mRNAs and supernatants were collected and subjected to qRT-PCR (for C) or
728
ELISA analysis (for D) to measure mRNA and protein expression of TNF-α and IL-6. Data
729
are presented as the mean ± SEM of four independent experiments. *P < 0.05, **P <0.01,
730
***P < 0.001.
M AN U
TE D
EP
731
SC
720
Fig.4. Comparison of MAPK activation in BMDMs infected with Mab WT or ∆esx.
733
A and B. Immunoblot analysis of whole-cell lysates from BMDMs infected with Mab WT or
734
∆esx (MOI = 5) for the indicated times (0-480 min) using antibodies against phosphorylated
735
forms of ERK, p38, and JNK. β-actin served as loading control. WB images representative of
736
three experiments are shown in panel A. Densitomety values for phospho-ERK, p-p38, and
737
p-JNK were normalized to β-actin (for B). Data are presented as the mean ± SEM of four
738
independent experiments. **P <0.01, ***P < 0.001.
739
C. Immunoblot analyses of BMDMs infected with Mab WT or ∆esx (MOI = 1, 5 or 10; for 30
AC C
732
ACCEPTED MANUSCRIPT 740
min) with antibodies raised to phosphorylated forms of ERK, p38, and JNK. β-actin served
741
as loading control. WB images representative of three experiments are shown.
742
Fig.5. Comparison of NF-κB signaling in BMDMs infected with Mab WT or ∆esx.
744
A and B. BMDMs were infected with Mab WT or ∆esx (MOI = 1, 5 or 10) for 30 min, followed
745
by immunostaining with anti-NF-κB p65 Ab, anti-rabbit-Alexa Fluor 488 (green), and DAPI to
746
visualize nuclei (blue). Representative immunofluorescence images (for A) and average
747
mean fluorescence intensity of cells exhibiting NF-κB nuclear translocation (for B) is shown.
748
C. Analysis of NF-κB p65 luciferase activity. BMDMs were transduced with adenovirus
749
carrying NF-κB luciferase reporter constructs for 36 h and infected with Mab WT or ∆esx
750
(MOI = 1, 5 or 10), or stimulated with LPS (100 ng/ml) for 6 h.
751
D. Immunoblot analysis of whole-cell lysates from BMDMs stimulated with Mab WT or ∆esx
752
(MOI = 5) for the indicated times (0-480 min) using antibodies against IκB-α. β-actin served
753
as a loading control. Data are presented as the mean ± SEM of four independent
754
experiments. *P < 0.05, ***P < 0.001.
755
TE D
M AN U
SC
RI PT
743
Fig.6. Purification and immunological characterization of EsxG▪EsxH in BMDMs during Mab
757
infection.
758
A. Multiple sequence alignments of conserved amino acids in EsxG (MAB_2229c, upper)
759
and EsxH (MAB_2228c, lower) ortholog from various mycobacterial strains (Mab, Mtb
760
H37Rv, Mtb H37Ra, M. bovis, M. ulcerans, M. leprae, M. smegmatis, and M. marinum).
761
B. Size-exclusion chromatography of rEsxGH complex. Mixture of purified EsxG and EsxH
762
proteins was injected onto Superdex 75 10/300 GL column. Elution peak corresponding to
763
EsxGH complex with a molecular weight of ~20 kDa is indicated.
764
C. SDS-PAGE analysis of eluted EsxG and EsxH proteins. Proteins were visualized by
765
Coomassie blue staining. M, mixture of purified EsxG and EsxH proteins. His-tagged EsxG
766
(upper arrow) and tag-free EsxH (lower arrow) are indicated, respectively.
AC C
EP
756
ACCEPTED MANUSCRIPT 767
D. BMDMs were treated with purified rEsxGH (5, 10 or 20 µg/ml, for 1 h), followed by
768
infection with ∆esx. They were then subjected to ELISA analysis to detect levels of TNF-α
769
and IL-6 at 18 h. Data are presented as the mean ± SEM of four independent experiments.
770
***P < 0.001.
RI PT
771
Supplementary figure 1. Construction of Mab mutants using recombineering system.
773
A and B. Schematic representation of genetic organization of esx-3 gene cluster in Mab WT
774
genome (for A) and gene disruption by zeocin cassette (for B). Position of oligonucleotides
775
(primer-F and primer-R) used for PCR validation and expected sizes of resulting amplicons
776
are indicated. C and D. ∆esx mutants were confirmed with primers shown (for C) and
777
individual gene deletions were analyzed with different primers (for D).
AC C
EP
TE D
M AN U
SC
772
RI PT
Figure 1.
B
SC
A
M AN U
2.0
esx WT
TE
D
1.0
0.0 0
12
24
36
48
60
Time (hours)
EP
0.5
72
84
AC C
OD600
1.5
96
AC C EP
TE
D
SC
M AN U
C D
RI PT
Figure 1.
AC C EP
TE
D
SC
M AN U
A
RI PT
Figure 2.
AC C EP
TE
D
SC
M AN U
B
RI PT
Figure 2.
C
AC C EP
TE
D
SC
M AN U
A B
RI PT
Figure 3.
AC C EP
TE
D
SC
M AN U
C D
RI PT
Figure 3.
AC C EP
TE
D
B
SC
M AN U
Figure 4.
RI PT
A
AC C EP
TE
D
C
SC
M AN U
RI PT
Figure 4.
AC C EP
TE
D
SC
M AN U
A B
RI PT
Figure 5.
C
AC C EP
TE
D
SC
D
M AN U
RI PT
Figure 5.
AC C EP
TE
D
RI PT
A
SC
M AN U
Figure 6.
AC C EP
TE
D
B
RI PT
C
SC
M AN U
Figure 6.
AC C EP
TE
D
RI PT
D
SC
M AN U
Figure 6.
S1286-4579(16)30123-X
DOI:
10.1016/j.micinf.2016.09.001
Reference:
MICINF 4426
To appear in:
Microbes and Infection
Received Date: 25 February 2016 Revised Date:
2 August 2016
Accepted Date: 5 September 2016
Please cite this article as: Y.S. Kim, C.-S. Yang, L.T. Nguyen, J.K. Kim, H.S. Jin, J.h. Choe, S.Y. Kim, H.-M. Lee, M. Jung, J.-M. Kim, M.H. Kim, E.-K. Jo, J.-C. Jang, Mycobacterium abscessus ESX-3 plays an important role in host inflammatory and pathological responses during infection, Microbes and Infection (2016), doi: 10.1016/j.micinf.2016.09.001. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
ACCEPTED MANUSCRIPT 1
Mycobacterium abscessus ESX-3 plays an important role in host inflammatory
2
and pathological responses during infection
3
Yi Sak Kim,1,3† Chul-Su Yang,4† Loi T. Nguyen,5 Jin Kyung Kim,1,3 Hyo Sun Jin,1,3 Jin
5
ho Choe,1,3 Soo Yeon Kim,1,3 Hye-Mi Lee,1,3 Mingyu Jung,2,3 Jin-Man Kim,2,3 Myung Hee
6
Kim,5 Eun-Kyeong Jo,1,3 and Ji-Chan Jang1,3,6*
7
RI PT
4
1
Department of Microbiology and 2Pathology, 3Department of Medical Science, College of
9
Medicine, Chungnam National University, Daejeon 301-747, Korea.
SC
8
4
Department of
Molecular and Life Science, Hanyang University, Ansan 426-791, Korea. 5Infection and
11
Immunity Research Center, Korea Research Institute of Bioscience and Biotechnology,
12
Daejeon 305-806, Korea. 6Molecular Mechanism of Antibiotics, Division of Life Science,
13
Research Institute of Life Science, Gyeongsang National University, Jinju, Gyeongnam,
14
Korea
18 19 20 21
TE D
17
EP
16
AC C
15
M AN U
10
*For correspondence. E-mail: [email protected];
22
Tel. (+82) (0)55 772 1368
23
† Both authors contributed equally to this work.
24
ACCEPTED MANUSCRIPT 25
Abstract Mycobacterial ESX systems are often related to pathogenesis during infection.
27
However, little is known about the function of ESX systems of Mycobacterium abscessus
28
(Mab). This study focuses on the Mab ESX-3 cluster, which contains major genes such as
29
esxH (Rv0288, low molecular weight protein antigen 7; CFP-7) and esxG (Rv0287, ESAT-6
30
like protein). An esx-3 (MAB 2224c-2234c)-deletional mutant of Mab (∆esx) was constructed
31
and used to infect murine and human macrophages. We then investigated whether Mab
32
∆esx modulated innate host immune responses in macrophages. Mab ∆esx infection
33
resulted in less pathological and inflammatory responses. Additionally, ∆esx resulted in
34
significantly decreased activation of inflammatory signaling and cytokine production in
35
macrophages compared to WT. Moreover, recombinant EsxG▪EsxH (rEsxGH) proteins
36
encoded by the ESX-3 region showed synergistic enhancement of inflammatory cytokine
37
generation in macrophages infected with ∆esx. Taken together, our data suggest that Mab
38
ESX-3 plays an important role in inflammatory and pathological responses during Mab
39
infection.
42 43 44 45
SC
M AN U
TE D EP
41
Keywords : Mycobacterium abscessus; ESX-3; host inflammation
AC C
40
RI PT
26
ACCEPTED MANUSCRIPT 46
1. Introduction Mycobacterium abscessus (hereafter referred to as Mab) is the most pathogenic strain
48
of the Mab complex, a group of rapidly growing non-tuberculous mycobacteria (NTM) and a
49
pathogenic mycobacterium [1]. Mab is commonly associated with a wide spectrum of human
50
diseases, including respiratory tract infections, traumatic skin and soft tissue infections,
51
bacteremia, and other infections involving almost all human organs [2,3,4]. Innate immunity
52
is a critical host defense system against mycobacterial infection that detects a variety of
53
mycobacterial-derived molecular patterns while inducing proinflammatory mediators and
54
antimicrobial proteins [5,6,7]. Numerous pattern-recognition receptors, such as Toll-like
55
receptors (TLRs), are involved in the recognition of mycobacterial products. These
56
mechanisms also trigger complex intracellular signaling activation, culminating in the
57
activation of nuclear factor (NF)-κB and mitogen-activated protein kinase (MAPK) signaling
58
in innate immune cells [8,9]. Activation of innate immune signaling leads to the production of
59
proinflammatory cytokines, including tumor necrosis factor TNF-α, interleukin (IL)-6, IL-1β,
60
and IL-12 [8,10].
TE D
M AN U
SC
RI PT
47
The development of molecular genetic approaches, such as whole-genome sequencing,
62
has markedly enhanced our understanding of various properties of Mab [11]. The
63
identification and immunological characterization of essential Mab genes contributes to the
64
development of novel protective and therapeutic strategies against Mab infection. However,
65
little is known about the function of many Mab genes in terms of their interactions with host
66
immune cells that elicit innate immune responses during Mab infection. In Mycobacterium
67
tuberculosis (Mtb), a widely characterized pathogen, five type VII secretion systems are
68
responsible for exporting proteins and members of the ESX family, which are involved in
69
tuberculosis pathogenesis and survival within host cells [12,13,14]. The early secreted
70
antigenic target of 6 kDa (ESAT-6)/culture filtrate protein of 10 kDa (CFP-10) complex,
71
secreted by the ESX-1 secretion system (also known as the RD1 region), plays an essential
AC C
EP
61
ACCEPTED MANUSCRIPT role in pathogenesis and immune activation during Mtb infection [15]. Furthermore, the ESX-
73
5 secretion system of pathogenic mycobacteria modulates the macrophage response in M.
74
marinum [16]. Compared to the ESX genomic location in Mtb, much less is known about the
75
immunological functions of the Mab ESX region. Mab only has two conserved ESX gene
76
clusters (ESX-3 and ESX-4) [17,18]. ESX-3 is conserved in all mycobacterial species [19]
77
and has a role in promoting mycobacterial virulence [20]. ESX-3 is also an essential
78
secretion system for iron and zinc homeostasis in M. tuberculosis and is consequently linked
79
to adaptations of M. tuberculosis in low zinc environments [21].Although this locus has been
80
implicated in mycobacterial growth [19], the function of ESX-3 has not been widely studied in
81
terms of host–pathogen interaction during Mab infection. Mab includes EsxG and EsxH
82
proteins, major proteins encoded by the esx-3 region, which show a high level of homology
83
with EsxG and EsxH from Mtb. The present study reports evidence showing an important
84
role for Mab ESX-3 in the induction of host immunopathological responses and increased
85
mycobacterial growth during infection.
89 90 91 92 93 94 95
SC
M AN U
TE D
88
EP
87
AC C
86
RI PT
72
ACCEPTED MANUSCRIPT 96
2. Material and Methods
97
2.1. Inactivation of esx gene cluster The mutation construct for the ESX-3 gene cluster was generated by PCR-
99
amplification from Mab ATCC 19977 genomic DNA as a template. The primer pair pJV531F
100
(CCCAAGCTTAGACCACTTCGCGGGCGACGG) and pJV531R (CTACCTGCAGCACTTAC
101
AGCCCTTCACCCG), including HindIII and PstI sites, respectively, was used to amplify
102
fragment 1, which consists of N-terminal amino acids together with a region ∼925 bp
103
downstream of Mab 2234c. Similarly, the primers pJV532F (CTACCTGCAGGTGCTGGG
104
GCGAGCACTTGC)
105
containing PstI and XbaI sites, respectively, were used for amplification of fragment 2 (1045
106
bp), which includes 140 bp of Mab 2224c. In more detail, fragment 1 was subcloned into
107
HindIII/PstI-digested pBluescript II SK(+) and fragment 2 was subsequently subcloned into
108
PstI/XbaI-digested pBluescript II SK(+) harboring fragment 1 to generate pBSK-∆esx. The
109
zeocin
110
(CTACCTGCAGCGCTAGCTCGAGCACGTGTTGACAATTAATCATCGGCATAGTATATC)
111
and ZeoR4pcD (CTAGCTGCAGATCTCGTAGCACGTGTCAGTC) from pcDNA3.1/Zeo(+). It
112
was digested with PstI, purified, and cloned into the PstI site of pBSK-∆esx to generate
113
pBSK-∆esx::zeo. Allelic-exchange substrate (AES) was amplified from pBSK-∆esx::zeo and
114
used to perform mutagenesis in Mab. The strain containing pJV53 was cultured and
115
incubated with 0.2% acetamide. Electrocompetent cells were prepared with ice-cold 10%
116
glycerol solution. The competent cells were electroporated with 100 ng of AES and plated on
117
50 µg/mL zeocin after 24 h of incubation at 37 °C. Muta tion events were verified by PCR and
118
sequencing.
(CGTCTAGAAGTGCCCTGCCCTCGCACGTC),
M AN U
was
pJV532R
amplified
using
two
different
primers,
Zeo-F2
AC C
EP
TE D
cassette
and
SC
RI PT
98
119 120
2.2. Bacteria culture condition, enumeration and In vitro growth kinetics
121 122
In vivo examinations were performed with Mab ATCC 19977; Wild-type (WT) and
ACCEPTED MANUSCRIPT 123
∆esx. Both strains were grown for 4 days, at 37°C, in M iddlebrook 7H9 broth supplemented
124
with albumin-dextrose-catalase (ADC, Difco) with daily agitation. These cultures were further
125
diluted serially (10-fold) to quantify colony-forming units (CFU)/mL.
126
spread on Middlebrook 7H10 agar media supplemented with 10% OADC (oleic acid, albumin,
127
dextrose and catalase, Difco) and incubated as described above until colonies were visible.
128
The visible Mab colonies were counted and adjusted based on the dilution factor. According
129
to this CFU determination, stocks of 1 × 108 CFU/mL were prepared and stored at -80°C until
130
used. Prior to infection, frozen stocks were thawed and 10-fold serial dilutions were prepared
131
in PBS plus 0.05% Tween-80 (PBST) before infection. To determine whether esx-3 gene
132
cluster disruption has brought in any change in the in vitro cultivation, we compared the
133
growth rates of Mab WT or ∆esx under enriched Middlebrook 7H9 broth supplemented with
134
10% ADC. A growth assay was performed in 3 mL shaking cultures at 37°C. The OD600 was
135
measured every 12 h for 4 days. All the experiments were performed in triplicate and
136
standard deviations were determined.
RI PT
M AN U
SC
2.3. Mice and cells
TE D
137 138
100 µL aliquots were
Wild-type female C57BL/6 mice (aged 6–8 weeks) were purchased from SAMTAKO
140
BIO (Gyeonggi-do, Korea) and were maintained under specific pathogen-free conditions. All
141
animal-related procedures were reviewed and approved by the Institutional Animal Care and
142
Use Committee, Chungnam National University School of Medicine (CNUH-014-A0008;
143
Daejeon, Korea). All animal procedures were conducted in accordance with guidelines of the
144
Korean Food and Drug Administration (KFDA). Murine bone marrow-derived macrophages
145
(BMDMs) were isolated and differentiated by growth for 4–5 days in medium containing
146
macrophage colony-stimulating factor (25 ng/mL; R&D Systems, 416-ML). The culture
147
medium was Dulbecco’s modified Eagle’s medium (DMEM; Lonza, 12-604F, NJ, USA),
148
which contained 10% FBS (Lonza, BW14-503E) and penicillin–streptomycin–amphotericin B
149
(Lonza, 17-745E). Human monocyte derived macrophages (MDMs) were prepared as
AC C
EP
139
ACCEPTED MANUSCRIPT 150
described previously [22]. Briefly, human monocytes were isolated from blood obtained from
151
healthy volunteers. The buffy coat was collected using a Ficoll gradient and monocytes were
152
enriched by adherence to tissue culture plastic. The Institutional Research and Ethics
153
Committee at Chungnam National University Hospital approved this study.
155
RI PT
154
2.4. Infection macrophages, mouse infection, histopathology, and bacterial counts
For infection, Mab WT and ∆esx were added to macrophages at 1:1 or 1:10
157
multiplicity of infection (MOI). After 4h of infection, extracellular mycobacteria were washed
158
out and infected macrophages were maintained in culture medium at 37°C and 5% CO 2 for 3
159
days. For bacterial burdens in the spleen and liver, mice per group were intravenously
160
infected with 1×107 CFU/mouse of Mab WT or ∆esx. Lungs, livers, and spleens were
161
harvested, and homogenates were counted at different times (1, 7, and 14 days) after
162
infection. For bacterial counting, the number of viable bacteria in each organ was determined
163
by plating serial dilutions of whole-organ homogenates on Middlebrook 7H10 agar
164
supplemented with OADC (Difco, Detroit, MI, USA). Colonies were counted after 3–5 days of
165
incubation at 37 °C, and the results were calculate d as the mean log10 CFU per organ.
166
Control mice were injected with PBST. For secretion of serum cytokine levels, 1×107 bacilli of
167
Mab WT or ∆esx were intravenously infected. ELISA was used to evaluate the levels of pro-
168
inflammatory cytokines, such as TNF-α and IL-6, in the infected lungs of mice within one day
169
post-infection. For IHC staining findings (for lung), groups of five mice each were
170
anaesthetized, their trachea exposed via a small midline incision. Each mice were infected
171
intratracheally with 5×105 CFU of Mab WT or ∆esx per mouse in 50 µL PBST. Lung samples
172
were fixed in 10% formalin and embedded in paraffin wax. Sections were then cut and
173
stained with hematoxylin and eosin. Inflammation in lung sections was graded for severity by
174
scanning multiple random fields in three sections of each tissue per mouse. An overall
175
histopathological score was assigned to each tissue in each animal based on the extent of
176
granulomatous inflammation as follows: 0 = no lesion, 1 = minimal lesion (1–10% of tissue in
AC C
EP
TE D
M AN U
SC
156
ACCEPTED MANUSCRIPT 177
section involved), 2 = mild lesion (11–30% involved), 3 = moderate lesion (30–50% involved),
178
4 = marked lesion (50–80% involved), and 5 = severe lesion (> 80% involved), as described
179
previously [20].
180
2.5. Reagents and antibodies Ultrapure lipopolysaccharide (LPS; tlrl-3pelps) was purchased from InvivoGen (San
182
Diego, USA). DAPI was purchased from Sigma. For western blotting, specific antibodies
183
(Abs) against phospho-SAPK/JNK (4668), phospho-p44/42 MAPK (ERK1/2) (9101), and
184
phospho-p38 MAP Kinase (9211) were obtained from Cell Signaling Technology (Beverly,
185
MA, USA). Anti-IκB-α (sc-371) and anti-actin (sc-1616) were obtained from Santa Cruz
186
Biotechnology (Santa Cruz, CA, USA). For IHC staining, paraffin wax-embedded lung
187
sections were stained using anti-COX2 (ab15191), anti-neutrophil (ab2557), and anti-iNOS
188
(ab3523) Abs biotin-conjugated rabbit anti-mouse IgG, as well as a peroxidase-conjugated
189
streptavidin Ab.
M AN U
SC
RI PT
181
190
2.6. RNA extraction, quantitative real-time PCR, enzyme-linked immunosorbent assays
192
(ELISA) and Western blotting
TE D
191
Total RNA was extracted from cells using the TRIzol reagent (Thermo Fisher
194
Scientific, 15596-026) according to the manufacturer’s protocol. Real-time PCR reactions
195
were performed according to the manufacturer’s instructions (SYBR green PCR master mix,
196
Qiagen), and thermal cycling was performed in a Rotor Gene 6000 instrument (Qiagen).
197
Primer sequences were as follows: mTNFα (forward: AGCACAGAAAGCATGAT
198
CCG, reverse: CTGATGAGAGGGAGGCCATT), mIL6 (forward: ACAAAGCCAGAGTCCTTC
199
AGA, reverse: TGGTCCTTAGCCACTCCTTC), mIL1β (forward: TGACGGACCCCAAAAGAT
200
GA, reverse: AAAGACACAGGTAGCTGCCA), mIL12p40 (forward: AGGTCACACTGGACCA
201
AAGG, reverse: TGGTTTGATGATGTCCCTGA), mβactin (forward: CCACCATGTACCCAGG
202
CATT, reverse: AGGGTGTAAAACGCAGCTCA), hTNFα (forward: GGCGTGGAGCTGAGAG
203
ATAAC, reverse: GGTGTGGGTGAGGAGCACAT), hIL6 (forward: TGTGAAAGCAGCAAAG
AC C
EP
193
ACCEPTED MANUSCRIPT AGGCACTG, reverse: ACAGCTCTGGCTTGTTCCTCACTA), and hβactin (forward: CACCAT
205
TGGCAATGAGCGGTTC, reverse: AGGTCTTTGCGGATGTCCACGT). In the sandwich
206
ELISA, serum and cell culture supernatants were analyzed using a Mouse BD OptEIA Set
207
ELISA Kit (BD Biosciences, USA) to detect TNF-α (558534), IL-6 (555240), IL-1β (559603),
208
and IL-12p40 (555165). The Human Ready-SET-Go ELISA kit (eBioscience, USA) was used
209
to detect TNF-α (88-7346) and IL-6 (88-7066). The limit of detection of the assay indicated
210
by the manufacturer (BD OptEIA Set ELISA Kit) was mouse 15 pg/ml (for mouse TNF-α), 4
211
pg/ml (for mouse IL-6, IL-1β, IL-12p40, and human TNF-α) and 2 pg/ml (for human IL-6). For
212
Western blotting, cell lysis was performed with RIPA buffer (50 mM Tris-HCl, pH 8.0, 150 mM
213
NaCl, 0.1% SDS, 1% NP-40, 0.5% deoxycholate and protease inhibitors) at 4 °C for 60 min.
214
The protein extracts were boiled in SDS sample buffer, loaded onto a 12% SDS-
215
polyacrylamide gel for electrophoresis, and transferred to a polyvinylidene difluoride
216
membrane (Millipore, IPVH00010). Signals were visualized with ECL solution (Millipore,
217
WBKL S0500) and detected with an UVitec Alliance mini-chemiluminescence device (UVitec,
218
Rugby, UK). The ImageJ software was used for densitometric analysis of the blots.
219
221
2.7. Immunofluorescence microscopy of NF-κB p65 translocation Translocation
of
NF-κBp65
EP
220
TE D
M AN U
SC
RI PT
204
into
the
nucleus
was
detected
using
immunofluorescence staining. Briefly, cells were infected with Mab WT or ∆esx for 30 min
223
and then fixed with 4% paraformaldehyde in PBS for 10 min. Cells were permeabilized with
224
0.25% Triton X-100 in PBS for 10 min and stained with anti-mouse NF-κB p65 (1:400, for 18
225
h at 4 °C; sc-372, Santa Cruz Biotechnology, Inc.) and anti-rabbit AlexaFluro 488 (1:400, for
226
2 h; A-11008, Invitrogen) at room temperature (RT). Nuclei were stained by incubation with
227
DAPI (Sigma) for 2 min. After mounting, fluorescence images were acquired using a
228
confocal laser-scanning microscope (LSM 710; Carl Zeiss, Jena, Germany).
AC C
222
229 230
2.8. NF-κB Luciferase reporter assays
ACCEPTED MANUSCRIPT Transduction with the NF-κB-Luciferase adenovirus (Genetransfer Vector Core;
232
Iowa City, IA, USA) was performed for 36 h, followed by infection with Mab WT or ∆esx for 6
233
h. Infected cells were washed three times in PBS, and cell extracts were prepared by adding
234
100 µL of 1× Passive Reporter Lysis Buffer (Promega, Madison, WI, USA). Luciferase
235
activity was measured using the Luciferase Assay System (Promega) according to the
236
manufacturer’s instructions.
RI PT
231
237
2.9. Recombinant protein purification
SC
238
The coding regions for EsxG (MAB_2229c) and EsxH (MAB_2228c) were subcloned
240
into NcoI and XhoI restriction sites of the pHis-parallel1 and pGST-parallel1 vectors,
241
respectively, containing recombinant TEV protease (rTEV) cleavage sites [24]. ClearColi
242
BL21 (DE3) cells (Lucigen, Middleton, USA) harboring each plasmid were grown in LB
243
medium containing ampicillin at 37 °C until they re ached an OD600 of 0.4–0.5. After cooling to
244
18 °C, protein expression was induced with 0.5 mM I PTG overnight. The cells expressing
245
each protein were then harvested and re-suspended in cooled buffer (50 mM Tris-HCl, pH
246
8.0, 300 mM NaCl, and 5% glycerol). The cell suspension was lysed with an ultra-high-
247
pressure homogenizer (UHPH; BEE International, USA). The expressed EsxG and EsxH
248
proteins were then purified by Ni-NTA agarose (Invitrogen, Carlsbad, CA) and GST agarose
249
(GE Healthcare, USA) affinity chromatography, respectively. GST-fused EsxH was further
250
purified by treatment with rTEV protease (Invitrogen) to remove GST and additional GST-
251
affinity chromatography. A complex of purified His-tagged EsxG and tag-free EsxH proteins
252
spontaneously formed upon mixing in a ratio of one to one. This complex was subjected to
253
size-exclusion chromatography for further purification. The complex protein was analyzed by
254
SDS-PAGE followed by Coomassie staining. Removal of endotoxin from recombinant
255
proteins was performed using polymyxin B-agarose (Sigma, USA) according to the
256
manufacturer’s protocol. Contamination with endotoxin was assessed with the Limulus
257
Amebocyte Lysate (LAL) QCL-1000 assay (Lonza, Walkersville, USA).
AC C
EP
TE D
M AN U
239
ACCEPTED MANUSCRIPT 258 259
2.10. Statistical Analyses All data obtained from independent experiments were analyzed by two-way analysis
261
of variance (ANOVA) with Bonferroni post-tests or one-way ANOVA with Bonferroni’s multiple
262
comparison test. Results are presented as the mean and standard error of the mean (SEM).
263
Differences were considered statistically significant when P < 0.05.
RI PT
260
264
3. Results
266
3.1. Construction of Mab mutants using a recombineering system
M AN U
SC
265
To study the functional role of ESX-3, recombineering was used to replace structural
268
gene regions with a zeocin cassette to provide resistance to zeocin [25]. Schematic
269
representations of the ESX-3 region genes in Mab WT and ∆esx mutant are shown in
270
Supplementary figure 1A and 1B, respectively. The resulting ∆esx strain was confirmed by
271
PCR using primers for the genomic region outside of the ESX-3 flanking regions. PCR
272
products (expected size 2.4 kb) would only be obtained if the zeocin cassette had been
273
inserted into the correct location on the chromosome. The expected PCR product size was
274
obtained from putative ∆esx; no product was obtained for WT Mab ATCC 19977 (13.7 kb;
275
Supplementary figure 1C). The amplicon was further analyzed by sequencing, which
276
confirmed the clear deletion of esx-3 regions from the genome (data not shown).
277
Furthermore, individual gene disruption was validated by PCR using individual gene-specific
278
primers (Supplementary figure 1D).
EP
AC C
279
TE D
267
280
3.2. Esx-3 locus is required for pathological changes during the acute phase of Mab infection
281
To determine whether esx-3 gene cluster disruption has brought in any change in the
282
in vitro cultivation, we compared the growth rates of Mab WT or ∆esx. Differences in growth
283
rate were compared using a nonparametric t test. As shown in Fig. 1A, the ∆esx did not
ACCEPTED MANUSCRIPT displayed a significantly reduced growth rate and doubling time compared to that of the Mab
285
WT. The mutant reached a stationary phase at 72 hours after inoculation with a similar
286
density compared to the WT (Fig. 1A, P=0.6270). Based on similarity of growth patterns
287
between Mab WT and ∆esx, we further assessed the role of esx-3 in Mab survival inside
288
macrophages. For this, survival of ∆esx was studied in BMDMs and compared with that of
289
Mab WT. The results showed that within 3 days, BMDMs were unable to eliminate the Mab
290
WT strain. As shown in Fig.1B, intracellular growth of Mab WT was significantly increased in
291
BMDMs compared with ∆esx at 3 days after infection. Similar findings were observed in data
292
from different MOIs (Fig.1B), suggesting that esx-3 is required for intracellular survival of
293
Mab. This finding was further studied using an in vivo acute model of infection. At days 7 and
294
14, the bacterial load in the spleen and liver was determined. As shown in Fig.1C,
295
significantly decreased splenic and hepatic bacillary loads were found in mice infected with
296
∆esx on day 7 after infection compared with those from mice infected with the WT strain. At
297
14 days post-infection, there were no change for bacterial growth in the livers of ∆esx
298
infected mice (Fig.1C). The results presented above show that growth of the ∆esx strain was
299
inhibited in mouse organs.
TE D
M AN U
SC
RI PT
284
To this end, we investigated whether mice infected with ∆esx and Mab WT strains
301
show different pathological responses. As shown in Fig.1D, the lungs of mice infected with
302
Mab WT exhibited extensive pathological changes at 7 days post-infection. In more detail,
303
the lung sections of mice infected with Mab WT exhibited severe lung pathology
304
characterized by much more dense alveolar spaces and increased granulomatous infiltrate.
305
However, significantly less granulomatous infiltrate was observed in ∆esx-infected animals.
306
Quantitative scoring of histopathological changes confirmed that the Mab WT group (n=5)
307
showed much more severe lung pathology than the ∆esx group at 7 days post-infection
308
(Fig.1D). Together, these pathological changes demonstrate that esx-3 influences the
309
pathogenesis of Mab in mice.
310
AC C
EP
300
ACCEPTED MANUSCRIPT 311
3.3. Mab ∆esx infection induces less inflammatory and pathological responses in vivo Mab vigorously activates innate immune responses in macrophages through
313
interactions between TLR2 and dectin-1 [26]. However, the role of the Mab esx-3 locus is not
314
well known in mice or macrophages. The serum levels of TNF-α and IL-6 in C57BL/6 mice
315
after infection were analyzed to examine if mice infected with ∆esx produced a more
316
attenuated inflammatory response than those infected with Mab WT. As shown in Fig.2A,
317
∆esx elicited a reduced amount of both TNF-α and IL-6 compared to the WT strain,
318
especially at one day post-infection.
SC
RI PT
312
319
Expression of cyclooxygenase 2 (COX2), inducible nitric oxide synthase (iNOS), and
321
neutrophils in lungs was further evaluated by immunohistochemistry. Immunoreactivity
322
against three antibodies (COX-2, iNOS, and neutrophil) was investigated in lung tissues
323
infected with Mab WT or ∆esx strains (Fig.2B and 2C). The amount of positively stained cells
324
was evaluated to calculate the percent of positive cells for scoring. As shown in Fig.2B,
325
COX-2, iNOS, and neutrophil staining in lung sections differed significantly between the
326
infected strains. Mab WT infected lung tissue samples showed >58% COX-2 and >79%
327
iNOS positive expression rates in immunohistochemical scoring (Fig.2C). In contrast, ∆esx
328
infected lung tissues showed lower positive rates for COX-2 (25%) and iNOS (52%)
329
expression. In addition, ∆esx infected lung tissues had lower rates of neutrophil infiltration
330
compared to those infected with Mab WT (Fig.2B and 2C). Together, these data suggest that
331
systemic and local inflammatory responses are markedly reduced in ∆esx-infected mice
332
compared with those of Mab WT-infected mice.
TE D
EP
AC C
333
M AN U
320
334
3.4. Mab ∆esx leads to less proinflammatory cytokine production in murine and human
335
macrophages compared to WT strain
336
The contribution of the ESX-3 region to pro-inflammatory responses was further
337
examined in murine and human macrophages. Proinflammatory cytokine generation was
ACCEPTED MANUSCRIPT compared for Mab WT- and ∆esx-infected BMDMs as well as human monocyte-derived
339
macrophages (MDMs). Mab WT robustly induced mRNA expression of proinflammatory
340
cytokines (TNF-α, IL-6, IL-1β, and IL-12 p40) from BMDMs after 3 h of infection. The mRNA
341
levels of proinflammatory cytokines induced by ∆esx were significantly lower than those
342
induced by Mab WT at different time points, as shown in Fig.3A. BMDMs infected with ∆esx
343
also produced smaller amounts of proinflammatory cytokines after 18 or 48 h of infection
344
compared to those infected with the Mab WT strain (Fig.3B).
SC
345
RI PT
338
The mRNA and protein expression of proinflammatory cytokines in human MDMs was
347
further examined after Mab WT or ∆esx infection. Similar to findings observed in murine
348
BMDMs, human MDMs tend to produce less TNF-α and IL-6 mRNA at different time points
349
(3 and 6 h for TNF-α; 6 and 18 h for IL-6; Fig.3C) in response to ∆esx than in response to
350
the WT strain. In addition, ∆esx infection produced smaller amounts of TNF-α and IL-6 in
351
MDMs at different time points (from 6 to 18 h for TNF-α; from 6 to 48 h for IL-6) compared to
352
Mab WT infection (Fig.3D). These results demonstrate that the ESX-3 region of Mab plays a
353
role in the induction of inflammatory responses in murine and human macrophages.
TE D
355
3.5. Mab ∆esx significantly attenuates activation of MAPK signaling in macrophages
EP
354
M AN U
346
The MAPK pathways play a key role in the host inflammatory response during
357
mycobacterial infection [27,28]. To examine the molecular mechanisms underlying ESX-3-
358
mediated inflammatory responses, the activation of ERK, p38, and JNK MAPKs in BMDMs
359
infected with either Mab WT or ∆esx was examined. As shown in Fig.4A, Mab WT robustly
360
activated three families of MAPKs in BMDMs after infection in a time-dependent manner. As
361
expected, the ∆esx-infected BMDMs showed less phosphorylation of ERK, p38, and JNK
362
MAPKs at different time points compared to WT-infected BMDMs (Fig.4A). Densitometric
363
analysis showed that the phosphorylation levels of ERK, p38, and JNK MAPKs were
364
significantly decreased in BMDMs infected with ∆esx at 15 to 60 mins post-infection
AC C
356
ACCEPTED MANUSCRIPT 365
compared to those infected with the WT strain (Fig.4B). Moreover, the ∆esx-induced
366
phosphorylation of ERK, p38, and JNK MAPKs was significantly decreased in BMDMs
367
compared with those infected by WT (Fig.4C). Taken together, these results suggest that the
368
ESX-3 region is associated with MAPK activation in BMDMs after infection.
RI PT
369 370
3.6. ESX-3 locus contributes to the activation of NF-κB signaling in macrophages during Mab
371
infection
We next examined whether the ESX-3 locus was involved in nuclear translocation and
373
activation of NF-κB, an essential transcriptional factor in inflammatory signaling [29], after
374
infection with ∆esx. Subcellular localization of NF-κB p65 in the nucleus was significantly
375
reduced in BMDMs infected with ∆esx compared to those infected with WT, as determined
376
by confocal microscopy after 30 min of infection (Fig.5A). This observation was further
377
analyzed by quantifying the effects of Mab WT and ∆esx on translocation of NF-κB/p65.
378
Quantification of cells from different fields showed a significantly lower percentage of NF-
379
κB/p65 translocation into nuclei in BMDMs infected with ∆esx compared with Mab WT
380
infection. Moreover, this relationship operated in a MOI-dependent manner (Fig.5B).
TE D
M AN U
SC
372
381
A NF-κB luciferase assay was also performed in BMDMs transduced with adenovirus
383
encoding a luciferase reporter plasmid containing response elements for NF-κB (Ad-NF-κB-
384
Luc). The activity of the NF-κB reporter gene was considerably reduced in BMDMs
385
transduced with Ad-NF-κB-Luc with ∆esx infection compared to those infected by Mab WT
386
(Fig.5C). As shown in Fig.5D, the effect of ∆esx on IκB-α degradation in BMDMs was also
387
examined. Degradation of IκB-α was prominent in BMDMs after 15-30 min of Mab WT
388
infection. However, few changes in IκB-α degradation were found in BMDMs after ∆esx
389
infection. Thus, the ESX-3 region enhanced activation of NF-κB signaling in BMDMs during
390
Mab infection.
391
AC C
EP
382
ACCEPTED MANUSCRIPT 392
3.7. rEsxGH protein is required for synergistic synthesis of TNF-α and IL-6 in BMDMs
393
infected with Mab ∆esx Previous studies have shown multiple sequence alignments highlighting the conservation
395
of amino acids in EsxG and EsxH orthologs from several mycobacterial strains, but not from
396
Mab [13]. We re-performed multiple sequence alignments of the conserved amino acids in
397
EsxG (MAB 2229c, upper) and EsxH (MAB 2228c, lower) orthologs from Mab, Mtb H37Rv,
398
Mtb H37Ra, M. bovis, M. ulcerans, M. leprae, M. smegmatis, and M. marinum (Fig.6A).
399
Overall, the amino acid sequences of orthologs were well conserved.
SC
RI PT
394
400
To evaluate the immunological relevance of both proteins, recombinant EsxGH (rEsxGH)
402
complex was purified. A previous study showed that the Mtb proteins CFP‐10 (Rv0287) and
403
ESAT‐6 (Rv0288), homologue proteins of EsxG and EsxH, respectively, form tight
404
heterodimeric complexes in the solution [30]. Consistent with the previous result, size-
405
exclusion chromatography analysis revealed that EsxG and EsxH proteins were co-eluted at
406
a fraction corresponding to the EsxGH complex with a molecular weight of ~20 kDa (Fig.6B).
407
The complex was confirmed by SDS-PAGE analysis (Fig.6C).
TE D
408
M AN U
401
Subsequently, BMDMs were stimulated in vitro with purified rEsxGH and then subjected
410
to endotoxin removal using polymyxin B-agarose. The cellular responses were analyzed and
411
compared with the response to Mab WT and ∆esx. As seen in Fig.6D, treatment of BMDMs
412
with rEsxGH protein alone did not induce the release of TNF-α or IL-6. Proinflammatory
413
cytokines were induced at a very low level of TNF-α and IL-6 from BMDMs infected with
414
∆esx, as seen in Fig.3. Interestingly, the production of TNF-α and IL-6 was synergistically
415
increased in ∆esx-infected BMDM when combined with rEsxGH protein in a dose-dependent
416
manner. These data suggest that rEsxGH from the ESX-3 region can rescue the function of
417
the ESX-3 region through in vitro complementation. Together, the EsxG and EsxH proteins
418
of the Mab ESX-3 region are associated with host inflammatory responses during the course
AC C
EP
409
ACCEPTED MANUSCRIPT 419
of Mab infection.
420 421 422
4. Discussion In this study, we characterized the innate immune function of the Mab ESX-3 region by
424
constructing an ESX-3 (MAB 2224c-2234c)-deletional mutant strain of Mab (∆esx) in murine
425
bone marrow-derived macrophages (BMDMs) and in vivo. Compared to Mab wild type (Mab
426
ATCC 19977), ∆esx infection resulted in induction of less histopathology and inflammatory
427
mediator production in vivo. It also resulted in lower levels of inflammatory signaling and
428
cytokine production in macrophages. Additionally, intracellular bacterial survival was
429
significantly attenuated in ∆esx-infected conditions. In vitro complementation with
430
recombinant EsxG▪EsxH (rEsxGH) proteins, two major proteins encoded by the ESX-3
431
region in Mab [13], was also performed. This showed that restoration of inflammatory
432
cytokine production was as likely as with the wild-type strain. The present study reports
433
evidence showing an important role for Mab ESX-3 in the induction of host
434
immunopathological responses and increased mycobacterial growth during infection.
SC
M AN U
TE D
435
RI PT
423
Mab is one of the most frequent causes of lung disease, accounting for around 80% of
437
pulmonary infections caused by rapidly growing mycobacteria [3]. One of the most serious
438
clinical burdens in an emerging Mab infection is chemotherapy difficulties, due to the intrinsic
439
drug resistance of Mab to various antibiotics [31]. There is an urgent need for the
440
development of new vaccines and therapeutic strategies to control Mab infection in both
441
immunocompetent and immunocompromized patients [32,33]. To this end, a more
442
comprehensive understanding of the host–pathogen interaction should be preceded by the
443
identification and functional characterization of essential Mab genes. Our findings identify the
444
Mab ESX-3 region as important for intracellular bacterial survival and elicitation of excessive
445
inflammatory and pathological responses during Mab infection.
AC C
EP
436
ACCEPTED MANUSCRIPT 446
In more detail, deletion of the Mab ESX-3 region leads to attenuated growth and
448
persistence in both macrophages. In addition, ∆esx infected organs such as spleen and liver
449
rapidly underwent a progressive reduction of CFU in comparison with wild-type strain at 7
450
days after infection. Mycobacterial virulence can be measured by the ability of bacteria to
451
invade, grow, and persist not only in macrophages, but also in an in vivo rodent model.
452
Sweeney et al. previously showed that the IKE (Mycobacterium smegmatis strain with
453
deletion of the esx-3 region) strain could not elicit different IL-6 amounts with parental and
454
∆esx-1 Msmeg. Fredric et al. also reported that Esx-1 deficient (∆RD1) M. marinum
455
appeared to perturb the host immune response [34]. In more detail, ∆RD1 M. marinum alters
456
the immune response by decreasing TNFα and IL-6 production. The presence of Esx-1
457
promotes NFκB activation in macrophages in vitro, which could account for increased TNFα
458
and IL-6 seen with infections by WT M. marinum in vivo. In this study, we observed innate
459
immune responses that were similar to those seen in the host immune response of ∆RD1 M.
460
marinum. This is because the Mab ESX-3 cluster harbors esxG (Rv0287, ESAT-6 like
461
protein), which has high homology with M. marinum esxG (MMAR 0546; ESAT-6 like protein)
462
(74% identities and 80% positives). The generation of proinflammatory cytokines (TNF-α, IL-
463
6, IL-1β, and IL-12p40) is significantly decreased by the ∆esx strain in macrophages from
464
mice and humans. This is the first report that Mab ESX-3 is involved in exacerbated
465
inflammatory responses, as well as disease pathology and reduced bacillary control, during
466
infection. TNF-α is a key proinflammatory cytokine that mediates mycobacterial killing, host
467
defense, chemokine expression, and granuloma formation [35,36]. However, excessive
468
levels of TNF-α can lead to detrimental effects in the host. For example, excessive secretion
469
of TNF-α has been implicated in clinical worsening and tissue damage, whereas TNF-α
470
reduction has been correlated with decreased granuloma size and necrosis [37]. Thus, the
471
appropriate induction and control of this cytokine are thought to be key in host-directed
472
responses against tuberculosis [38]. Our report suggests that the Mab esx-3 region is
AC C
EP
TE D
M AN U
SC
RI PT
447
ACCEPTED MANUSCRIPT 473
involved in serum cytokine production that subsequently influences virulence in a mouse
474
model of infection.
475
Inflammatory responses triggered by mycobacterial infection lead to the robust
477
activation of intracellular signaling cascades involving three subfamilies of MAPKs and NF-
478
κB activation [8,26]. We also found that macrophage inflammatory signaling (NF-κB and
479
MAPK) is markedly downregulated by ∆esx infection. Indeed, there have been many reports
480
of in vitro and in vivo immune-modulating activity of the ESAT-6 antigen of Mtb. The ESAT-6
481
antigen elicited vaccine-enhancing Th17 immune responses through TLR2/MyD88 signaling
482
[39]. In contrast, RD-1 region antigens played the key role of down-regulating the functions
483
of macrophages, potentially contributing to Mtb virulence [40]. Previous studies also showed
484
that disruption of the M. marinum PPE38 gene resulted in reduced levels of TNF-α and IL-6
485
secretion in infected macrophages [41]. BLAST analysis revealed that MAB_2230c within
486
the ESX-3 gene cluster shares intermediate homology (~35%) with M. marinum PPE38
487
(data not shown). Taken together, our data suggest that the ESX-3 region may contribute to
488
excessive inflammatory responses and signaling activation in host macrophages.
SC
M AN U
TE D
489
RI PT
476
Efficiently mounting host defenses against mycobacterial infection depends on both
491
restriction of bacterial replication and prevention of overwhelming inflammatory responses
492
[42]. The immunopathological responses to Mab are poorly characterized compared to the
493
widely studied Mtb infection. The name “Mab” originated from abscess formation during
494
infection [43]. Clinical manifestations of Mab infection are often related to abscess
495
formations that require surgical treatment and severe inflammatory responses, such as
496
ulcerative, abscess-forming lesions [44,45]. In this study, we report that Mab infection
497
resulted in markedly increased granulomatous infiltrate and inflammatory infiltrates in mouse
498
lungs. We also found that the infiltration of neutrophils and immune cells expressing COX-2
499
and iNOS was markedly increased in mouse tissues within 1 week of infection with the Mab
AC C
EP
490
ACCEPTED MANUSCRIPT WT strain. Notably, pathological responses found in Mab WT-infected lungs and other
501
tissues were significantly attenuated compared to those from ∆esx-infected mice. These
502
data indicate that the Mab ESX-3 region is important in Mab pathogenesis and virulence
503
during infection.
RI PT
500
504
In this study, we were unable to complement the Mab WT strain with a mutant strain
506
given the current genetic tools. As with the M. smegmatis IKE strain, we could not
507
complement with cosmid pYUB1336, which harbors an intact M. tuberculosis ESX-3 locus
508
(Rv0282–Rv0292) [20]. We speculate that we would have been unable to complement Esx-3
509
function in an M. smegmatis mutant even if it were expressed pYUB1336 in this species,
510
suggesting that esx-3 functions are species-specific. Other E. coli/ Mycobacterial expression
511
vectors using the hsp60 promoter fused with the ESX-3 region (MAB 2224c-2234c) were
512
also unable to complement, probably due to overexpression of a gene cluster with several
513
membrane proteins. To compensate for this in an alternative way, recombinant proteins
514
rEsxG and rEsxH were generated from esxH and esxH genes, which were expected to be
515
the main functional genes in the Mab ESX-3 region. The ∆esx phenotype was partly rescued
516
when ∆esx was co-incubated with rEsxG and rEsxH. Although the recombinant protein alone
517
was unable to induce proinflammatory cytokine release, ∆esx - rEsxG and rEsxH could elicit
518
a dose-dependent increase in TNF-α and IL-6 levels in macrophages to levels observed in
519
Mab WT strain-infected cells. Recent studies showed that Mtb type VII effector EsxH, in
520
complex with EsxG, is involved in impaired phagosomal maturation by disrupting the
521
endosomal sorting complex required for transport (ESCRT) function, restricting intracellular
522
bacterial growth [46]. Combined with our data, this suggests that at least two proteins, esxG
523
and esxH gene products, may contribute to the pathological responses induced by the Mab
524
ESX-3 region. Further studies are needed to clarify the distinct function of each gene located
525
within the ESX-3 region of the Mab genome.
AC C
EP
TE D
M AN U
SC
505
ACCEPTED MANUSCRIPT 526
In summary, we report a function of the Mab ESX-3 cluster with regard to virulence and
528
replication failure in a mouse model of infection. The absence of Mab ∆esx resulted in less
529
accumulation of neutrophils and inflammatory mediator release in vivo. Furthermore, Mab
530
ESX-3 plays an important role in excessive proinflammatory cytokine production through
531
modulation of MAPKs and NF-κB in macrophages. The EsxGH proteins of the Mab ESX-3
532
region contributed to a rescue of the attenuated inflammatory responses induced by the
533
∆esx strain. The immunopathological action of the Mab ESX-3 region may be associated
534
with Mab virulence and inflammatory responses during the course of Mab infection.
SC
RI PT
527
536
M AN U
535
Acknowledgements
We thank D. M. Shin and J. J. Kim for helpful discussion and reagents. We thank D.
538
Ray for critical reading of the manuscript. This work was supported by a grant of the Korea
539
Health Technology R&D Project through the Korea Health Industry Development Institute
540
(KHIDI), by the National Research Foundation of Korea (NRF) grant funded by the Korean
541
government (MSIP) (2011-0030049) at Hanyang University, and by the Basic Science
542
Research Program through the NRF funded by the Ministry of Education (NRF-
543
2014R1A6A1029617) .
545 546 547 548 549 550
EP
AC C
544
TE D
537
Conflict of interest
No conflict of interest
ACCEPTED MANUSCRIPT References
552
[1] Field SK, Cowie RL. Lung disease due to the more common nontuberculous
553
mycobacteria. Chest 2006; 129:1653-72.
554
[2] Brown-Elliott BA, Wallace RJ Jr. Clinical and taxonomic status of pathogenic
555
nonpigmented or late-pigmenting rapidly growing mycobacteria. Clin Microbiol Rev
556
2002;15:716-46.
557
[3] Griffith DE, Aksamit T, Brown-Elliott BA, Catanzaro A, Daley C, Gordin F, et al. An official
558
ATS/IDSA statement: diagnosis, treatment, and prevention of nontuberculous mycobacterial
559
diseases. Am J Respir Crit Care Med 2007;175:367-416.
560
[4] Nessar R, Cambau E, Reyrat JM, Murray A, Gicquel B. Mycobacterium abscessus: a new
561
antibiotic nightmare. J Antimicrob Chemother 2012;67:810-8.
562
[5] Thoma-Uszynski S, Stenger S, Takeuchi O, Ochoa MT, Engele M, Sieling PA, et al.
563
Induction of direct antimicrobial activity through mammalian toll-like receptors. Science
564
2001;291:1544-7.
565
[6] Yamashiro LH, Oliveira SC, Báfica A. Innate immune sensing of nucleic acids from
566
mycobacteria. Microbes Infect 2014;16:991-7.
567
[7] Stamm CE, Collins AC, Shiloh MU. Sensing of Mycobacterium tuberculosis and
568
consequences to both host and bacillus. Immunol Rev 2015;264:204-19.
569
[8] Basu J, Shin DM, Jo EK. Mycobacterial signaling through toll-like receptors. Front Cell
570
Infect Microbiol 2012;2:145.
571
[9] Killick KE, Ní Cheallaigh C, O'Farrelly C, Hokamp K, MacHugh DE, Harris J. Receptor-
572
mediated recognition of mycobacterial pathogens. Cell Microbiol 2013;15:1484-95.
573
[10] Hossain MM, Norazmi MN. Pattern recognition receptors and cytokines in
574
Mycobacterium
575
2013;2013:179174.
576
[11] Howard ST. Recent progress towards understanding genetic variation in the
577
Mycobacterium abscessus complex. Tuberculosis (Edinb) 2013;93:S15-20.
AC C
EP
TE D
M AN U
SC
RI PT
551
tuberculosis
infection--the
double-edged
sword?
Biomed
Res
Int
ACCEPTED MANUSCRIPT [12] Stanley SA, Raghavan S, Hwang WW, Cox JS. Acute infection and macrophage
579
subversion by Mycobacterium tuberculosis require a specialized secretion system. Proc Natl
580
Acad Sci USA 2003;100:13001-6.
581
[13] Ilghari D, Lightbody KL, Veverka V, Waters LC, Muskett FW, Renshaw PS, et al.
582
Solution structure of the Mycobacterium tuberculosis EsxG.EsxH complex: functional
583
implications and comparisons with other M. tuberculosis Esx family complexes. J Biol Chem
584
2011;286:29993-30002.
585
[14] Liu W, Peng Y, Yin Y, Zhou Z, Zhou W, Dai Y. The involvement of NADPH oxidase-
586
mediated ROS in cytokine secretion from macrophages induced by Mycobacterium
587
tuberculosis ESAT-6. Inflammation 2014;37:880-92.
588
[15] Lewis KN, Liao R, Guinn KM, Hickey MJ, Smith S, Behr MA, et al. Deletion of RD1 from
589
Mycobacterium tuberculosis mimics bacille Calmette-Guérin attenuation. J Infect Dis
590
2003;187:117-23.
591
[16] Abdallah AM, Savage ND, van Zon M, Wilson L, Vandenbroucke-Grauls CM, van der
592
Wel NN, et al. The ESX-5 secretion system of Mycobacterium marinum modulates the
593
macrophage response. J Immunol 2008;181:7166-75.
594
[17] Choo SW, Wee WY, Ngeow YF, Mitchell W, Tan JL, Wong GJ, et al. Genomic
595
reconnaissance of clinical isolates of emerging human pathogen Mycobacterium abscessus
596
reveals high evolutionary potential. Sci Rep 2014;4:4061.
597
[18] Sassi M, Drancourt M. Genome analysis reveals three genomospecies in
598
Mycobacterium abscessus. BMC Genomics. 2014;15:359.
599
[19] Siegrist MS, Unnikrishnan M, McConnell MJ, Borowsky M, Cheng TY, Siddiqi N, et al.
600
Mycobacterial Esx-3 is required for mycobactin-mediated iron acquisition. Proc Natl Acad Sci
601
USA 2009;106:18792-7.
602
[20] Sweeney KA, Dao DN, Goldberg MF, Hsu T, Venkataswamy MM, Henao-Tamayo M, et
603
al. A recombinant Mycobacterium smegmatis induces potent bactericidal immunity against
604
Mycobacterium tuberculosis. Nat Med 2011;17:1261-8.
AC C
EP
TE D
M AN U
SC
RI PT
578
ACCEPTED MANUSCRIPT [21] Serafini A, Pisu D, Palù G, Rodriguez GM, Manganelli R. The ESX-3 secretion system is
606
necessary for iron and zinc homeostasis in Mycobacterium tuberculosis. PLoS One.
607
2013;8:e78351.
608
[22] Yang CS, Shin DM, Kim KH, Lee ZW, Lee CH, Park SG, et al. NADPH oxidase 2
609
interaction with TLR2 is required for efficient innate immune responses to mycobacteria via
610
cathelicidin expression. J Immunol 2009;182:3696-705.
611
[23] Wang J, Li BX, Ge PP, Li J, Wang Q, Gao GF, Qiu XB, Liu CH. Mycobacterium
612
tuberculosis suppresses innate immunity by coopting the host ubiquitin system. Nat Immunol.
613
2015;16:237-45.
614
[24] Sheffield P, Garrard S, Derewenda Z. Overcoming expression and purification problems
615
of RhoGDI using a family of "parallel" expression vectors. Protein Expr Purif 1999;15:34-9.
616
[25] van Kessel JC, Marinelli LJ, Hatfull GF. Recombineering mycobacteria and their phages.
617
Nat Rev Microbiol 2008;6:851-7.
618
[26] Shin DM, Yang CS, Yuk JM, Lee JY, Kim KH, Shin SJ, et al. Mycobacterium abscessus
619
activates the macrophage innate immune response via a physical and functional interaction
620
between TLR2 and dectin-1. Cell Microbiol 2008;10:1608-21.
621
[27] Zhou B, He Y, Zhang X, Xu J, Luo Y, Wang Y, et al. Targeting mycobacterium protein
622
tyrosine phosphatase B for antituberculosis agents. Proc Natl Acad Sci USA 2010;107:4573-
623
8.
624
[28] Seto S, Tsujimura K, Koide Y. Coronin-1a inhibits autophagosome formation around
625
Mycobacterium tuberculosis-containing phagosomes and assists mycobacterial survival in
626
macrophages. Cell Microbiol 2012;14:710-27.
627
[29] Kim TS1, Kim YS, Yoo H, Park YK, Jo EK. Mycobacterium massiliense induces
628
inflammatory responses in macrophages through Toll-like receptor 2 and c-Jun N-terminal
629
kinase. J Clin Immunol 2014;34:212-23.
630
[30] Renshaw PS, Lightbody KL, Veverka V, Muskett FW, Kelly G, Frenkiel TA, et al.
631
Structure and function of the complex formed by the tuberculosis virulence factors CFP-10
AC C
EP
TE D
M AN U
SC
RI PT
605
ACCEPTED MANUSCRIPT and ESAT-6. EMBO J 2005;24:2491-8.
633
[31] Lee MR, Sheng WH, Hung CC, Yu CJ, Lee LN, Hsueh PR. Mycobacterium abscessus
634
complex infections in humans. Emerg Infect Dis 2015;21:1638-46.
635
[32] Oh CT, Moon C, Park OK, Kwon SH, Jang J. Novel drug combination for
636
Mycobacterium abscessus disease therapy identified in a Drosophila infection model. J
637
Antimicrob Chemother 2014;69:1599-1607.
638
[33] Abdalla MY, Switzer BL, Goss CH, Aitken ML, Singh PK, Britigan BE. Gallium
639
compounds exhibit potential as new therapeutic agents against Mycobacterium abscessus.
640
Antimicrob Agents Chemother 2015;59: 4826-34.
641
[34] Carlsson F, Kim J, Dumitru C, Barck KH, Carano RA, Sun M, et al. Host-detrimental role
642
of Esx-1-mediated inflammasome activation in mycobacterial infection. PLoS Pathog.
643
2010;6:e1000895.
644
[35] Bermudez LE, Young LS. Tumor necrosis factor, alone or in combination with IL-2, but
645
not IFN-gamma, is associated with macrophage killing of Mycobacterium avium complex. J
646
Immunol 1988;140:3006-13.
647
[36] Flynn JL, Goldstein MM, Chan J, Triebold KJ, Pfeffer K, Lowenstein CJ, et al. Tumor
648
necrosis factor-alpha is required in the protective immune response against Mycobacterium
649
tuberculosis in mice. Immunity 1995;2:561-72.
650
[37] Bekker LG, Moreira AL, Bergtold A, Freeman S, Ryffel B, Kaplan G. Immunopathologic
651
effects of tumor necrosis factor alpha in murine mycobacterial infection are dose dependent.
652
Infect Immun 2000;68:6954-61.
653
[38] Dorhoi A, Kaufmann SH. Tumor necrosis factor alpha in mycobacterial infection. Semin
654
Immunol 2014;26:203-209.
655
[39] Chatterjee S, Dwivedi VP, Singh Y, Siddiqui I, Sharma P, Van Kaer L, et al. Early
656
secreted antigen ESAT-6 of Mycobacterium tuberculosis promotes protective T helper 17
657
cell responses in a toll-like receptor-2-dependent manner. PLoS Pathog 2011;7:e1002378.
658
[40] Pathak SK, Basu S, Basu KK, Banerjee A, Pathak S, Bhattacharyya A, et al. Direct
AC C
EP
TE D
M AN U
SC
RI PT
632
ACCEPTED MANUSCRIPT extracellular interaction between the early secreted antigen ESAT-6 of Mycobacterium
660
tuberculosis and TLR2 inhibits TLR signaling in macrophages. Nat Immunol 2007;8:610-8.
661
[41] Dong D, Wang D, Li M, Wang H, Yu J, Wang C, et al. PPE38 modulates the innate
662
immune response and is required for Mycobacterium marinum virulence. Infect Immun
663
2012;80:43-54.
664
[42] Nandi B, Behar SM. Regulation of neutrophils by interferon-γ limits lung inflammation
665
during tuberculosis infection. J Exp Med. 2011;208:2251-62.
666
[43] Moore M, Frerichs JB. An unusual acid-fast infection of the knee with subcutaneous,
667
abscess-like lesions of the gluteal region; report of a case with a study of the organism,
668
Mycobacterium abscessus, n. sp. J Invest Dermatol 1953;20:133-169.
669
[44] Song JY, Sohn JW, Jeong HW, Cheong HJ, Kim WJ, Kim MJ. An outbreak of post-
670
acupuncture cutaneous infection due to Mycobacterium abscessus. BMC Infect Dis 2006;6:6.
671
[45] Johnson MM, Odell JA. Nontuberculous mycobacterial pulmonary infections. J Thorac
672
Dis 2014;6:210-20.
673
[46] Mehra A, Zahra A, Thompson V, Sirisaengtaksin N, Wells A, Porto M, et al.
674
Mycobacterium tuberculosis type VII secreted effector EsxH targets host ESCRT to impair
675
trafficking. PLoS Pathog 2013;9:e100373.
676
.
679 680 681 682 683 684 685
SC
M AN U
TE D
EP
678
AC C
677
RI PT
659
ACCEPTED MANUSCRIPT 686
Figure legends
687
Fig.1. Mab esx-3 gene cluster is required for in vitro and in vivo growth.
689
A. Mab WT and ∆esx were grown in enriched Middlebrook 7H9 broth supplemented with
690
0.05% Tween and ADC and OD value was taken every 12 h at 600 nm. All data was
691
repeated in triplicates.
692
B. BMDMs were infected with different MOI (MOI of 1 or 10) of both either Mab WT or ∆esx,
693
washed, and macrophage lysates plated for CFU counts on 7H10 agar.
694
C. C57BL/6 mice were intravenously infected with 1×107 CFU of Mab WT and ∆esx strains.
695
Bacillary loads were determined in spleens and livers of C57BL/6 (n = 5) infected with Mab
696
WT and ∆esx at 1, 7, and 14 days post-infection. All data points are represented by log10
697
CFU values, and bars indicate standard errors.
698
D. Comparison of histopathological findings from C57BL/6 mice were intratracheally infected
699
with 5×105 CFU of Mab WT and ∆esx strains or PBST mock control. The figure depicts a
700
representative photograph of the extent of pathological damage of mice infected with PBST
701
mock control (n = 3), Mab WT (n = 5), and ∆esx (n = 5) at 7 days post-infection. Quantitative
702
scoring of histopathology is shown in the left lower panel. Data are presented as the mean ±
703
SEM of four independent experiments. *P < 0.05, **P <0.01, ***P < 0.001. Scale bars, 100
704
µm.
SC
M AN U
TE D
EP
AC C
705
RI PT
688
706
Fig.2. Esx-3 disruption induces less pro-inflammatory responses in vivo.
707
A. Blood serum levels of pro-inflammatory cytokines such as TNF-α (left) and IL-6 (right)
708
were measured by ELISA analysis from C57BL/6 mice were intravenously infected with
709
1×107 CFU of Mab WT and ∆esx strains (n = 9).
710
B. Expression of COX-2 and iNOS, as well as neutrophil infiltration in lung tissues from
711
C57BL/6 mice were intratracheally infected with 5×105 CFU of Mab WT (n = 5) and ∆esx
712
strains (n = 5) or PBST mock control (n = 3) at 7 days post-infection. Representative results
ACCEPTED MANUSCRIPT of immunohistochemistric analysis of expression of COX-2 and iNOS, and neutrophil
714
infiltration in lung tissues from mice infected with Mab WT or ∆esx (left). A brown color
715
indicates positive staining for the indicted proteins. Scale bars, 100 µm (for COX2 and iNOS)
716
or 50 µm (for Neutrophil).
717
C. Quantitative scoring of histopathologic findings (for B) by percentage of positively strained
718
cells. *P < 0.05, **P <0.01, ***P < 0.001.
719
RI PT
713
Fig.3. Proinflammatory cytokine generation in murine and human macrophages after
721
infection with Mab WT or ∆esx strain.
722
A and B. BMDMs were infected with Mab WT or ∆esx (MOI = 5) for the indicated times. The
723
mRNAs and supernatants were collected and subjected to qRT-PCR (for A) or ELISA
724
analysis (for B) to measure mRNA and protein expression of TNF-α, IL-6, IL-1β, and IL-
725
12p40.
726
C and D. Human MDMs were infected with Mab WT or ∆esx (MOI = 5) for the indicated
727
times. The mRNAs and supernatants were collected and subjected to qRT-PCR (for C) or
728
ELISA analysis (for D) to measure mRNA and protein expression of TNF-α and IL-6. Data
729
are presented as the mean ± SEM of four independent experiments. *P < 0.05, **P <0.01,
730
***P < 0.001.
M AN U
TE D
EP
731
SC
720
Fig.4. Comparison of MAPK activation in BMDMs infected with Mab WT or ∆esx.
733
A and B. Immunoblot analysis of whole-cell lysates from BMDMs infected with Mab WT or
734
∆esx (MOI = 5) for the indicated times (0-480 min) using antibodies against phosphorylated
735
forms of ERK, p38, and JNK. β-actin served as loading control. WB images representative of
736
three experiments are shown in panel A. Densitomety values for phospho-ERK, p-p38, and
737
p-JNK were normalized to β-actin (for B). Data are presented as the mean ± SEM of four
738
independent experiments. **P <0.01, ***P < 0.001.
739
C. Immunoblot analyses of BMDMs infected with Mab WT or ∆esx (MOI = 1, 5 or 10; for 30
AC C
732
ACCEPTED MANUSCRIPT 740
min) with antibodies raised to phosphorylated forms of ERK, p38, and JNK. β-actin served
741
as loading control. WB images representative of three experiments are shown.
742
Fig.5. Comparison of NF-κB signaling in BMDMs infected with Mab WT or ∆esx.
744
A and B. BMDMs were infected with Mab WT or ∆esx (MOI = 1, 5 or 10) for 30 min, followed
745
by immunostaining with anti-NF-κB p65 Ab, anti-rabbit-Alexa Fluor 488 (green), and DAPI to
746
visualize nuclei (blue). Representative immunofluorescence images (for A) and average
747
mean fluorescence intensity of cells exhibiting NF-κB nuclear translocation (for B) is shown.
748
C. Analysis of NF-κB p65 luciferase activity. BMDMs were transduced with adenovirus
749
carrying NF-κB luciferase reporter constructs for 36 h and infected with Mab WT or ∆esx
750
(MOI = 1, 5 or 10), or stimulated with LPS (100 ng/ml) for 6 h.
751
D. Immunoblot analysis of whole-cell lysates from BMDMs stimulated with Mab WT or ∆esx
752
(MOI = 5) for the indicated times (0-480 min) using antibodies against IκB-α. β-actin served
753
as a loading control. Data are presented as the mean ± SEM of four independent
754
experiments. *P < 0.05, ***P < 0.001.
755
TE D
M AN U
SC
RI PT
743
Fig.6. Purification and immunological characterization of EsxG▪EsxH in BMDMs during Mab
757
infection.
758
A. Multiple sequence alignments of conserved amino acids in EsxG (MAB_2229c, upper)
759
and EsxH (MAB_2228c, lower) ortholog from various mycobacterial strains (Mab, Mtb
760
H37Rv, Mtb H37Ra, M. bovis, M. ulcerans, M. leprae, M. smegmatis, and M. marinum).
761
B. Size-exclusion chromatography of rEsxGH complex. Mixture of purified EsxG and EsxH
762
proteins was injected onto Superdex 75 10/300 GL column. Elution peak corresponding to
763
EsxGH complex with a molecular weight of ~20 kDa is indicated.
764
C. SDS-PAGE analysis of eluted EsxG and EsxH proteins. Proteins were visualized by
765
Coomassie blue staining. M, mixture of purified EsxG and EsxH proteins. His-tagged EsxG
766
(upper arrow) and tag-free EsxH (lower arrow) are indicated, respectively.
AC C
EP
756
ACCEPTED MANUSCRIPT 767
D. BMDMs were treated with purified rEsxGH (5, 10 or 20 µg/ml, for 1 h), followed by
768
infection with ∆esx. They were then subjected to ELISA analysis to detect levels of TNF-α
769
and IL-6 at 18 h. Data are presented as the mean ± SEM of four independent experiments.
770
***P < 0.001.
RI PT
771
Supplementary figure 1. Construction of Mab mutants using recombineering system.
773
A and B. Schematic representation of genetic organization of esx-3 gene cluster in Mab WT
774
genome (for A) and gene disruption by zeocin cassette (for B). Position of oligonucleotides
775
(primer-F and primer-R) used for PCR validation and expected sizes of resulting amplicons
776
are indicated. C and D. ∆esx mutants were confirmed with primers shown (for C) and
777
individual gene deletions were analyzed with different primers (for D).
AC C
EP
TE D
M AN U
SC
772
RI PT
Figure 1.
B
SC
A
M AN U
2.0
esx WT
TE
D
1.0
0.0 0
12
24
36
48
60
Time (hours)
EP
0.5
72
84
AC C
OD600
1.5
96
AC C EP
TE
D
SC
M AN U
C D
RI PT
Figure 1.
AC C EP
TE
D
SC
M AN U
A
RI PT
Figure 2.
AC C EP
TE
D
SC
M AN U
B
RI PT
Figure 2.
C
AC C EP
TE
D
SC
M AN U
A B
RI PT
Figure 3.
AC C EP
TE
D
SC
M AN U
C D
RI PT
Figure 3.
AC C EP
TE
D
B
SC
M AN U
Figure 4.
RI PT
A
AC C EP
TE
D
C
SC
M AN U
RI PT
Figure 4.
AC C EP
TE
D
SC
M AN U
A B
RI PT
Figure 5.
C
AC C EP
TE
D
SC
D
M AN U
RI PT
Figure 5.
AC C EP
TE
D
RI PT
A
SC
M AN U
Figure 6.
AC C EP
TE
D
B
RI PT
C
SC
M AN U
Figure 6.
AC C EP
TE
D
RI PT
D
SC
M AN U
Figure 6.