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Mutations in the gyrA and parC genes associated with fluoroquinolone resistance in clinical isolates of Citrobacter freundii
FEMS Microbiology Letters 154 (1997) 409^414
Mutations in the gyrA and parC genes associated with £uoroquinolone resistance in clinical isolates of Citrobacter freundii
Yoshinori Nishino, Takashi Deguchi, Mitsuru Yasuda, Takeshi Kawamura, Masahiro Nakano, Emiko Kanematsu, Shigehiko Ozeki, Yukimichi Kawada * Department of Urology, Gifu University School of Medicine, Gifu 500, Japan
Received 3 June 1997; revised 23 July 1997; accepted 28 July 1997
Abstract
We determined partial sequences of the gyrA and parC genes of Citrobacter freundii type strain, and then examined 38 C. clinical strains isolated from patients with urinary tract infections for the association of alterations in GyrA and ParC with susceptibility to fluoroquinolones. Our results suggest that in C. freundii DNA gyrase may be a primary target of quinolones, that an amino acid change at Thr-83 or Asp-87 in GyrA is sufficient to decrease susceptibility to fluoroquinolones, and that accumulation of changes in GyrA with the simultaneous presence of an alteration at Ser-80 or Glu-84 in ParC may be associated with the development of high-level fluoroquinolone resistance in C. freundii clinical isolates. freundii
Keywords : Citrobacter freundii
; DNA gyrase; Topoisomerase IV
1. Introduction
Neisseria gonorrhoeae, and Haemo, alterations in the GyrA subunit of DNA gyrase play a primary role in developing quinolone resistance [5^9]. In these species, alterations in the ParC subunit of DNA topoisomerase IV play a complementary role in increasing quinolone resistance [7,9^12]. In C. freundii, however, the mechanisms of quinolone resistance have not been well studied. In the present study, we attempted to amplify the gyrA and parC genes of C. freundii, corresponding to the quinolone resistance-determining region (QRDR), and then we analyzed clinical strains of C. freundii isolated from patients with urinary tract infections for the association of alterations of GyrA and ParC with quinolone resistance. Escherichia coli
,
philus in£uenzae
Citrobacter freundii is often isolated from patients with urinary tract infections. Fluoroquinolones, which have a good activity against C. freundii, have been e¡ective in curing urinary tract infections with this pathogen [1]. However, we have found an increase in the number of C. freundii isolates with decreased susceptibilities to £uoroquinolones. Recently, several mechanisms of quinolone resistance have been identi¢ed in some bacterial species [2^4]. In Gram-negative bacterial species, such as
* Corresponding author. Tel: +81 (58) 265 1241; Fax: +8 (58) 265 9009.
0378-1097 / 97 / $17.00 ß 1997 Federation of European Microbiological Societies. Published by Elsevier Science B.V. PII S 0 3 7 8 - 1 0 9 7 ( 9 7 ) 0 0 3 6 1 - 3
FEMSLE 7789 25-10-97
Y. Nishino et al. / FEMS Microbiology Letters 154 (1997) 409^414
410
Japan), an inoculum of 10
2. Materials and methods
4
CFU per spot was ap-
plied to agar plates containing serial 2-fold dilutions
2.1. Bacterial strains
of each drug. MICs were de¢ned as the lowest concentrations of drug that completely inhibited visible
C. freundii
Type strain of
ATCC8090 was pur-
chased from the American Type Culture Collection.
C. freundii
Thirty-eight clinical strains of
growth of the inoculum after incubation for 18 h at 37³C.
used in this
study were isolated from 1991 through 1994 from Japanese patients with urinary tract infection and
2.4. Detection of mutations in the gyrA and parC genes
maintained in our laboratory. To avoid testing multiple isolates from a single patient,
C. freundii
was
Thirty-eight clinical strains were examined for the
gyrA
and
parC
isolated in only one urinary culture from each pa-
presence of mutations in the
tient during the infection period and was used for
For analysis of the mutations in the region corre-
genes.
this study. No patients were given any quinolones
sponding to the QRDR of the
when they visited a clinic.
parC
E. coli gyrA
and
genes, DNA fragments were ampli¢ed using
the following two sets of primers, EC-GYRA-A
2.2. Determination of partial sequences of the C. freundii gyrA and parC genes
and
EC-GYRA-B,
and
EC-PARC-A
and
EC-
PARC-B, and sequencing of PCR products was performed by procedures similar to those previously re-
For partial sequencing of the regions of the and
parC
genes of
C. freundii
gyrA
analogous to the QRDR of the
E. coli gyrA
gene,
DNA fragments were ampli¢ed from the chromosomal DNA of type strain by polymerase chain reaction (PCR) with two sets of primers, EC-GYRA-A and EC-GYRA-B for EC-PARC-B for
parC,
gyrA,
ported [8,10].
containing the region
2.5. Case study of a £uoroquinolone treatment failure in urinary tract infection with emergence of a post-treatment isolate with enhanced resistance to £uoroquinolones
and EC-PARC-A and
and the PCR products were
We examined clinical strains that were isolated
sequenced. EC-GYRA-A (5P-CGCGTACTTTACG-
from a case of £uoroquinolone treatment failure in
CCATGAACGTA-3P) and EC-GYRA-B (5P-CAG-
urinary tract infection. A 65 year-old Japanese man
ACGGATTTCCGTATAACGC-3P)
with urethral stricture presented at the clinic with
were
located
C. freundii
within the consensus amino acids of the bacterial
dysuria and urinary turbidity. A strain of
GyrA proteins and were identical to nucleotide posi-
7 (named GU-CF08) was isolated from his urine (10
E. coli gyrA
CFU/ml). He was treated with a novel £uoroquino-
gene [5]. EC-PARC-A (5P-CTGAACGCCAGCGC-
lone, AM-1155 [13], 100 mg, twice daily for 7 days.
GAAATT-3P) and EC-PARC-B (5P-GCGAAAGA-
When
TTTGGGATCGTC-3P) were identical to nucleotide
symptoms,
tions 139 to 162 and 360 to 381 of the
positions 185 to 204 and 353 to 372 of the
parC
he
returned a
to
strain
of
the
clinic
with
C. freundii
continuing
(named
E. coli
GU7 CF09) was isolated again (10 CFU/ml). To assess
gene [3]. DNA extraction, PCR ampli¢cation,
whether the pre- and post-treatment isolates were
and sequencing of the PCR products were performed
isogenic, arbitrarily primed PCR analysis was per-
as reported previously [8].
formed [14], and biochemical characteristics were examined
2.3. MIC testing
by
Dickinson
using Co.,
Enterotube
Tokyo,
II
Japan).
(Nippon
Becton
The
strains
two
were tested for the MICs of cipro£oxacin, nor£oxaThe susceptibilities of the strains to cipro£oxacin
cin, AM-1155, piperacillin, cefazolin, cefotaxime, ce-
and nor£oxacin were determined by the 2-fold agar
¢xime, aztreonam, imipenem, gentamicin, chloram-
dilution method. The strains were cultured overnight
phenicol,
in Mueller-Hinton broth at 37³C, and using an in-
examined for the presence of mutations in the
oculator (Microplanter ; Sakura Seisakusho, Tokyo,
and
parC
FEMSLE 7789 25-10-97
and
tetracycline.
They
were
also
gyrA
genes. The analysis of the mutations and
Y. Nishino et al. / FEMS Microbiology Letters 154 (1997) 409^414
411
susceptibilities were performed in the manner identical to that described above. 2.6. Statistical analysis
Statistical analysis was conducted using the Wilcoxon rank sum test. All statistical comparisons were two-tailed and were performed with the signi¢cance set at P 6 0.05. 2.7. Nucleotide sequence accession number
The partial sequence of the C. freundii gyrA and gene reported here appears in the DDBJ, EMBL, and GenBank nucleotide sequence databases with the accession numbers AB003913 and AB003914, respectively. parC
Fig. 2. Comparisons of particular regions of the nucleotide sequence of the DNA fragment ampli¢ed from the chromosomal DNA of C. freundii ATCC 8090 (CfparC) with the equivalent region of E. coli (EcoparC) and of the deduced amino acid sequence (CfParC) with the equivalent regions of E. coli (EcoParC). Portions of the primers are excluded from the sequence. Dashes on the lines of EcoparC and EcoParC indicate nucleotides and amino acids identical to nucleotides in CfparC and amino acids in CfParC, respectively. 3. Results and discussion
3.1. Ampli¢cation of the C. freundii gyrA and parC genes
Fig. 1. Comparisons of particular regions of the nucleotide sequence of the DNA fragment ampli¢ed from the chromosomal DNA of C. freundii ATCC 8090 (CfgyrA) with the equivalent region of E. coli (EcogyrA) and of the deduced amino acid sequence (CfGyrA) with the equivalent regions of E. coli (EcoGyrA). Portions of the primers are excluded from the sequence. Dashes on the lines of EcogyrA and EcoGyrA indicate nucleotides and amino acids identical to nucleotides in CfgyrA and amino acids in CfGyrA, respectively.
The primers EC-GYRA-A and EC-GYRA-B ampli¢ed a DNA fragment of the expected 243 bp from the chromosomal DNA of type strain of C. freundii. The PCR product was sequenced, and the nucleotide sequence and amino acid sequence of the C. freundii gyrA gene and GyrA protein are shown in Fig. 1. The determined nucleotide sequence of a 197 bp DNA fragment excluding the primers showed 87.3% similarity with the corresponding region of the gyrA gene of E. coli. The deduced 64 amino acid sequence showed 98.5% identity with the GyrA protein of E. coli and exhibited 60 to 82% identities with the corresponding regions of other bacterial GyrA proteins [8,15,16]. Conversely, the primers EC-PARC-A and EC-PARC-B ampli¢ed a DNA fragment of the expected 188 bp from the chromosomal DNA of type strain of C. freundii. The 148 bp DNA fragment excluding the primers exhibited 93.3% identity with the corresponding regions of the parC gene of E. coli. The deduced 49 amino acid sequence was identical to that of the
FEMSLE 7789 25-10-97
412
Y. Nishino et al. / FEMS Microbiology Letters 154 (1997) 409^414
ParC protein of E. coli (Fig. 2) and exhibited 51 to 69% identities with the regions of the Neisseria gonorrhoeae ParC and Staphylococcus aureus GrlA proteins, respectively [7,17]. From these ¢ndings, we concluded that the determined sequences were partial sequences of the C. freundii gyrA and parC genes. 3.2. Detection of mutations in the gyrA and parC genes ampli¢ed from clinical isolates of C. freundii
The association of mutations in gyrA and parC genes with susceptibilities to £uoroquinolones was determined in 38 urinary tract-derived clinical strains of C. freundii. In 17 isolates with both cipro£oxacin and nor£oxacin MICs of 1.56 mg/l, the nucleotide sequences in the regions of the gyrA and parC genes analyzed in this study contained no mutations resulting in amino acid changes in GyrA and ParC proteins (Table 1). Seven strains with a cipro£oxacin MIC of 6.25 mg/l and nor£oxacin MICs of 12.5 mg/l to 25 mg/l had single mutations in the gyrA gene alone, resulting in an amino acid change of
Thr-83CIle. Six strains with cipro£oxacin MICs of 12.5 mg/l to 25 mg/l and nor£oxacin MICs of 25 mg/ l to 50 mg/l had single mutations in the gyrA and parC genes. Eight strains with cipro£oxacin MICs of 50 mg/l to 200 mg/l and nor£oxacin MICs of 100 mg/l to 200 mg/l had double mutations in the gyrA gene and single mutations in the parC gene. All the mutations observed in codon 83 of the gyrA gene were C-to-T substitutions, generating an amino acid change of Thr-83CIle. The mutations in codon 87 were G-to-A, G-to-C, and A-to-C substitutions, resulting in amino acid changes of Asp-87CAsn, Asp-87CTyr, and Asp-87CVal, respectively. All the mutations in the codons of the parC gene corresponding to Ser-80 and Glu-84 of the E. coli ParC protein were a G-to-T substitutions, generating Ser80CIle. All the mutations in the codon corresponding to Glu-84 of the E. coli ParC protein were G-toA substitutions, resulting in Glu-84CLys. These alterations observed in GyrA and ParC of C. freundii were analogous to those that were frequently found to be responsible for £uoroquinolone resistance in E. coli and other bacterial species [6,7,12,15^17]. In this study, we found no strains having alterations in
Table 1 Alterations in GyrA and ParC and susceptibilities to cipro£oxacin and nor£oxacin in clinical isolates of C. freundii MIC (mg/l) Amino acid change a a NFLX CPFX GyrA ParC Strain 83 87 80 Type strain 90.025 90.025 Thr(ACC) Asp(GAC) Ser(AGC) ^ ^ 01,11,66 0.1 0.05 ^b 12,58 0.2 0.05 ^ ^ ^ 60,69 0.2 0.1 ^ ^ ^ 04,15 0.78 0.39 ^ ^ ^ 03,07 0.78 0.78 ^ ^ ^ 10,19,65,67 1.56 0.78 ^ ^ ^ 59,68 1.56 1.56 ^ ^ ^ 71,72,73 12.5 6.25 Ile(ATC) ^ ^ 05,06,23,70 25 6.25 Ile(ATC) ^ ^ 02 25 12.5 Ile(ATC) ^ ^ 36 25 12.5 Ile(ATC) ^ Ile(ATC) 34,35 25 25 Ile(ATC) ^ ^ 16,29 50 25 Ile(ATC) ^ Ile(ATC) 18 100 50 Ile(ATC) Tyr(TAC) Ile(ATC) 31,48,51 100 50 Ile(ATC) Tyr(TAC) ^ 55 100 100 Ile(ATC) Tyr(TAC) Ile(ATC) 13,49,50 200 200 Ile(ATC) Val(GTC) Ile(ATC) a NFLX, nor£oxacin; CPFX, cipro£oxacin. b ^, identical to type strain.
FEMSLE 7789 25-10-97
84 Glu(GAA) ^ ^ ^ ^ ^ ^ ^ ^ ^ Lys(AAA) ^ Lys(AAA) ^ ^ Lys(AAA) ^ ^
Y. Nishino et al. / FEMS Microbiology Letters 154 (1997) 409^414
413
Table 2 Antimicrobial susceptibility pro¢les and alterations in GyrA and ParC of pre- and post-treatment
C. freundii
strains isolated from a case
of £uoroquinolone treatment failure in urinary tract infection MICs and alterations
Pre-treatment isolate GU-CF08
Post-treatment isolate GU-CF09
Nor£oxacin
25
100
Cipro£oxacin
12.5
50
O£oxacin
25
50
MIC (mg/l) of :
AM-1155
6.25
Piperacillin
6.25
25 6.25
Cefazolin
3.13
3.13
Cefotaxime
0.78
0.78
Ce¢xime
3.13
3.13
Aztreonam
1.56
1.56
Imipenem
0.2
0.2
Gentamicin
0.39
0.39
Chloramphenicol
0.78
0.78
Tetracycline
3.13
3.13
Alterations in : GyrA
C C
Thr-83
ParC
Ser-80
Ile
C C C
Thr-83
Asp-87
Ile
Ser-80
Ile Asn
Ile
ParC without the simultaneous presence of altera-
tical to each other. These analyses suggested that the
tions in GyrA.
pre- and post-treatment isolates were isogenic. For
The strains having a single or double amino acid
these strains, Table 2 shows the antimicrobial sus-
change in GyrA exhibited signi¢cantly higher-level
ceptibilities and amino acid changes in GyrA and
resistance
ParC. The isolate GU-CF08 exhibited 4-fold higher
to
cipro£oxacin
and
nor£oxacin
than
those without alterations in either GyrA or ParC
MICs
(P
0.01). The six strains with single amino acid
showed MICs of the other agents identical to those
changes in GyrA and ParC were signi¢cantly more
of GU-CF08. In the isolate GU-CF08, the threonine
resistant to cipro£oxacin and nor£oxacin than the
at position 83 was changed into an isoleucine in the
seven strains with a single amino acid change in
GyrA, and the serine at position 80 was substituted
6
GyrA
P
6
alone
(cipro£oxacin,
P
6
0.05 ;
nor£oxacin,
0.01). The eight strains with a double amino
of
£uoroquinolones
than
GU-CF09,
but
C
with an isoleucine in ParC. In the isolate GU-CF09, an alteration of Asp-87
Asn in GyrA was observed
acid change in GyrA and a single amino acid change
in addition to the amino acid changes in GyrA and
in ParC were signi¢cantly more resistant to cipro-
ParC identical to those found in the isolate GU-
£oxacin and nor£oxacin than the six strains with
CF08. The accumulation of amino acid changes in
single
GyrA appeared to contribute to a speci¢c increase in
(P
6
amino
acid
changes
in
GyrA
and
ParC
0.01).
£uoroquinolone resistance in the isolate GU-CF09. In this study, we determined the association of
3.3. Case study of a £uoroquinolone treatment failure in urinary tract infection caused by a quinolone-resistant C. freundii strain
mutations in
gyrA
and
parC
genes with susceptibil-
ities to £uoroquinolones, and reported a case study of a £uoroquinolone treatment failure in an urinary tract infection, accompanied with emergence of a
The electrophoresis pro¢le of the DNAs ampli¢ed
post-treatment isolate with enhanced resistance to
by AP-PCR from the post-treatment isolate GU-
£uoroquinolones. Although we have not proved the
CF09 was identical to that from the pre-treatment
alterations in GyrA and ParC actually cause the re-
isolate GU-CF08. The biochemical characteristics of
sistance phenotype, the ¢ndings of this study do sug-
the pre- and post-treatment isolates also were iden-
gest, in
FEMSLE 7789 25-10-97
C. freundii
as well as in
E. coli
and
N. go-
Y. Nishino et al. / FEMS Microbiology Letters 154 (1997) 409^414
414
norrhoeae,
that DNA gyrase is a primary target of
quinolones, that only a single amino acid change at Thr-83 in GyrA is su¤cient to generate high-level resistance
to
cipro£oxacin
and
nor£oxacin,
and
gyrA and parC in £uoroquinolone-resistant isolates.
regions of
Mol. Microbiol. 14, 371^380. [8] Deguchi, T., Yasuda, M., Asano, M., Tada, K., Iwata, H., Komeda, H., Ezaki, T., Saito, I. and Kawada, Y. (1995) DNA gyrase mutations in quinolone-resistant clinical isolates of
that the accumulation of amino acid changes in
Neisseria gonorrhoeae.
GyrA with the simultaneous presence of alterations
561^563.
in ParC contributes to increment in cipro£oxacin and nor£oxacin resistance [8^10]. To our knowledge, this is the ¢rst report to identify the mutations in the
gyrA
parC
and
genes associated with £uoroquino-
lone resistance in clinical isolates of
C. freundii.
This study should provide useful information for understanding the molecular mechanisms of £uoroquinolone resistance in
C. freundii.
Antimicrob. Agents Chemother. 39,
[9] Georgiou, M., Munoz, R., Roman, F., Canton, R., GomezLus, R., Campos, J. and De la Campa, A.G. (1996) Cipro£oxacin-resistant
Hemophilus in£uenzae
strains possess muta-
tions in analogous positions GyrA and ParC. Antimicrob. Agents Chemother. 40, 1741^1744. [10] Deguchi, T., Yasuda, M., Nakano, M., Ozeki, S., Ezaki, T., Saito, I. and Kawada, Y. (1996) Quinolone-resistant
gonorrhoeae ;
Neisseria
Correlation of alterations in the GyrA subunit
of DNA gyrase and the ParC subunit of topoisomerase IV with antimicrobial susceptibility pro¢les. Antimicrob. Agents Chemother. 40, 1020^1023. [11] Vila, J., Ruiz, J., Goni, P. and Jimenez de Anta, M.T. (1996)
Acknowledgments
parC in quinolone-resistant clinical Escherichia coli. Antimicrob. Agents Chemother.
Detection of mutations in isolates of
40, 491^493.
The authors thank Ms. Kyoko Hirata for technical assistance and laboratory analysis.
[12] Kumagai, Y., Kato, J-I., Hoshino, K., Akasaka, T., Sato, K. and Ikeda, H. (1996) Quinolone-resistant mutants of
chia coli
DNA topoisomerase IV
parC
Escheri-
gene. Antimicrob.
Agents Chemother. 40, 710^714.
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acquires mutations in analogous
FEMSLE 7789 25-10-97
Mutations in the gyrA and parC genes associated with £uoroquinolone resistance in clinical isolates of Citrobacter freundii
Yoshinori Nishino, Takashi Deguchi, Mitsuru Yasuda, Takeshi Kawamura, Masahiro Nakano, Emiko Kanematsu, Shigehiko Ozeki, Yukimichi Kawada * Department of Urology, Gifu University School of Medicine, Gifu 500, Japan
Received 3 June 1997; revised 23 July 1997; accepted 28 July 1997
Abstract
We determined partial sequences of the gyrA and parC genes of Citrobacter freundii type strain, and then examined 38 C. clinical strains isolated from patients with urinary tract infections for the association of alterations in GyrA and ParC with susceptibility to fluoroquinolones. Our results suggest that in C. freundii DNA gyrase may be a primary target of quinolones, that an amino acid change at Thr-83 or Asp-87 in GyrA is sufficient to decrease susceptibility to fluoroquinolones, and that accumulation of changes in GyrA with the simultaneous presence of an alteration at Ser-80 or Glu-84 in ParC may be associated with the development of high-level fluoroquinolone resistance in C. freundii clinical isolates. freundii
Keywords : Citrobacter freundii
; DNA gyrase; Topoisomerase IV
1. Introduction
Neisseria gonorrhoeae, and Haemo, alterations in the GyrA subunit of DNA gyrase play a primary role in developing quinolone resistance [5^9]. In these species, alterations in the ParC subunit of DNA topoisomerase IV play a complementary role in increasing quinolone resistance [7,9^12]. In C. freundii, however, the mechanisms of quinolone resistance have not been well studied. In the present study, we attempted to amplify the gyrA and parC genes of C. freundii, corresponding to the quinolone resistance-determining region (QRDR), and then we analyzed clinical strains of C. freundii isolated from patients with urinary tract infections for the association of alterations of GyrA and ParC with quinolone resistance. Escherichia coli
,
philus in£uenzae
Citrobacter freundii is often isolated from patients with urinary tract infections. Fluoroquinolones, which have a good activity against C. freundii, have been e¡ective in curing urinary tract infections with this pathogen [1]. However, we have found an increase in the number of C. freundii isolates with decreased susceptibilities to £uoroquinolones. Recently, several mechanisms of quinolone resistance have been identi¢ed in some bacterial species [2^4]. In Gram-negative bacterial species, such as
* Corresponding author. Tel: +81 (58) 265 1241; Fax: +8 (58) 265 9009.
0378-1097 / 97 / $17.00 ß 1997 Federation of European Microbiological Societies. Published by Elsevier Science B.V. PII S 0 3 7 8 - 1 0 9 7 ( 9 7 ) 0 0 3 6 1 - 3
FEMSLE 7789 25-10-97
Y. Nishino et al. / FEMS Microbiology Letters 154 (1997) 409^414
410
Japan), an inoculum of 10
2. Materials and methods
4
CFU per spot was ap-
plied to agar plates containing serial 2-fold dilutions
2.1. Bacterial strains
of each drug. MICs were de¢ned as the lowest concentrations of drug that completely inhibited visible
C. freundii
Type strain of
ATCC8090 was pur-
chased from the American Type Culture Collection.
C. freundii
Thirty-eight clinical strains of
growth of the inoculum after incubation for 18 h at 37³C.
used in this
study were isolated from 1991 through 1994 from Japanese patients with urinary tract infection and
2.4. Detection of mutations in the gyrA and parC genes
maintained in our laboratory. To avoid testing multiple isolates from a single patient,
C. freundii
was
Thirty-eight clinical strains were examined for the
gyrA
and
parC
isolated in only one urinary culture from each pa-
presence of mutations in the
tient during the infection period and was used for
For analysis of the mutations in the region corre-
genes.
this study. No patients were given any quinolones
sponding to the QRDR of the
when they visited a clinic.
parC
E. coli gyrA
and
genes, DNA fragments were ampli¢ed using
the following two sets of primers, EC-GYRA-A
2.2. Determination of partial sequences of the C. freundii gyrA and parC genes
and
EC-GYRA-B,
and
EC-PARC-A
and
EC-
PARC-B, and sequencing of PCR products was performed by procedures similar to those previously re-
For partial sequencing of the regions of the and
parC
genes of
C. freundii
gyrA
analogous to the QRDR of the
E. coli gyrA
gene,
DNA fragments were ampli¢ed from the chromosomal DNA of type strain by polymerase chain reaction (PCR) with two sets of primers, EC-GYRA-A and EC-GYRA-B for EC-PARC-B for
parC,
gyrA,
ported [8,10].
containing the region
2.5. Case study of a £uoroquinolone treatment failure in urinary tract infection with emergence of a post-treatment isolate with enhanced resistance to £uoroquinolones
and EC-PARC-A and
and the PCR products were
We examined clinical strains that were isolated
sequenced. EC-GYRA-A (5P-CGCGTACTTTACG-
from a case of £uoroquinolone treatment failure in
CCATGAACGTA-3P) and EC-GYRA-B (5P-CAG-
urinary tract infection. A 65 year-old Japanese man
ACGGATTTCCGTATAACGC-3P)
with urethral stricture presented at the clinic with
were
located
C. freundii
within the consensus amino acids of the bacterial
dysuria and urinary turbidity. A strain of
GyrA proteins and were identical to nucleotide posi-
7 (named GU-CF08) was isolated from his urine (10
E. coli gyrA
CFU/ml). He was treated with a novel £uoroquino-
gene [5]. EC-PARC-A (5P-CTGAACGCCAGCGC-
lone, AM-1155 [13], 100 mg, twice daily for 7 days.
GAAATT-3P) and EC-PARC-B (5P-GCGAAAGA-
When
TTTGGGATCGTC-3P) were identical to nucleotide
symptoms,
tions 139 to 162 and 360 to 381 of the
positions 185 to 204 and 353 to 372 of the
parC
he
returned a
to
strain
of
the
clinic
with
C. freundii
continuing
(named
E. coli
GU7 CF09) was isolated again (10 CFU/ml). To assess
gene [3]. DNA extraction, PCR ampli¢cation,
whether the pre- and post-treatment isolates were
and sequencing of the PCR products were performed
isogenic, arbitrarily primed PCR analysis was per-
as reported previously [8].
formed [14], and biochemical characteristics were examined
2.3. MIC testing
by
Dickinson
using Co.,
Enterotube
Tokyo,
II
Japan).
(Nippon
Becton
The
strains
two
were tested for the MICs of cipro£oxacin, nor£oxaThe susceptibilities of the strains to cipro£oxacin
cin, AM-1155, piperacillin, cefazolin, cefotaxime, ce-
and nor£oxacin were determined by the 2-fold agar
¢xime, aztreonam, imipenem, gentamicin, chloram-
dilution method. The strains were cultured overnight
phenicol,
in Mueller-Hinton broth at 37³C, and using an in-
examined for the presence of mutations in the
oculator (Microplanter ; Sakura Seisakusho, Tokyo,
and
parC
FEMSLE 7789 25-10-97
and
tetracycline.
They
were
also
gyrA
genes. The analysis of the mutations and
Y. Nishino et al. / FEMS Microbiology Letters 154 (1997) 409^414
411
susceptibilities were performed in the manner identical to that described above. 2.6. Statistical analysis
Statistical analysis was conducted using the Wilcoxon rank sum test. All statistical comparisons were two-tailed and were performed with the signi¢cance set at P 6 0.05. 2.7. Nucleotide sequence accession number
The partial sequence of the C. freundii gyrA and gene reported here appears in the DDBJ, EMBL, and GenBank nucleotide sequence databases with the accession numbers AB003913 and AB003914, respectively. parC
Fig. 2. Comparisons of particular regions of the nucleotide sequence of the DNA fragment ampli¢ed from the chromosomal DNA of C. freundii ATCC 8090 (CfparC) with the equivalent region of E. coli (EcoparC) and of the deduced amino acid sequence (CfParC) with the equivalent regions of E. coli (EcoParC). Portions of the primers are excluded from the sequence. Dashes on the lines of EcoparC and EcoParC indicate nucleotides and amino acids identical to nucleotides in CfparC and amino acids in CfParC, respectively. 3. Results and discussion
3.1. Ampli¢cation of the C. freundii gyrA and parC genes
Fig. 1. Comparisons of particular regions of the nucleotide sequence of the DNA fragment ampli¢ed from the chromosomal DNA of C. freundii ATCC 8090 (CfgyrA) with the equivalent region of E. coli (EcogyrA) and of the deduced amino acid sequence (CfGyrA) with the equivalent regions of E. coli (EcoGyrA). Portions of the primers are excluded from the sequence. Dashes on the lines of EcogyrA and EcoGyrA indicate nucleotides and amino acids identical to nucleotides in CfgyrA and amino acids in CfGyrA, respectively.
The primers EC-GYRA-A and EC-GYRA-B ampli¢ed a DNA fragment of the expected 243 bp from the chromosomal DNA of type strain of C. freundii. The PCR product was sequenced, and the nucleotide sequence and amino acid sequence of the C. freundii gyrA gene and GyrA protein are shown in Fig. 1. The determined nucleotide sequence of a 197 bp DNA fragment excluding the primers showed 87.3% similarity with the corresponding region of the gyrA gene of E. coli. The deduced 64 amino acid sequence showed 98.5% identity with the GyrA protein of E. coli and exhibited 60 to 82% identities with the corresponding regions of other bacterial GyrA proteins [8,15,16]. Conversely, the primers EC-PARC-A and EC-PARC-B ampli¢ed a DNA fragment of the expected 188 bp from the chromosomal DNA of type strain of C. freundii. The 148 bp DNA fragment excluding the primers exhibited 93.3% identity with the corresponding regions of the parC gene of E. coli. The deduced 49 amino acid sequence was identical to that of the
FEMSLE 7789 25-10-97
412
Y. Nishino et al. / FEMS Microbiology Letters 154 (1997) 409^414
ParC protein of E. coli (Fig. 2) and exhibited 51 to 69% identities with the regions of the Neisseria gonorrhoeae ParC and Staphylococcus aureus GrlA proteins, respectively [7,17]. From these ¢ndings, we concluded that the determined sequences were partial sequences of the C. freundii gyrA and parC genes. 3.2. Detection of mutations in the gyrA and parC genes ampli¢ed from clinical isolates of C. freundii
The association of mutations in gyrA and parC genes with susceptibilities to £uoroquinolones was determined in 38 urinary tract-derived clinical strains of C. freundii. In 17 isolates with both cipro£oxacin and nor£oxacin MICs of 1.56 mg/l, the nucleotide sequences in the regions of the gyrA and parC genes analyzed in this study contained no mutations resulting in amino acid changes in GyrA and ParC proteins (Table 1). Seven strains with a cipro£oxacin MIC of 6.25 mg/l and nor£oxacin MICs of 12.5 mg/l to 25 mg/l had single mutations in the gyrA gene alone, resulting in an amino acid change of
Thr-83CIle. Six strains with cipro£oxacin MICs of 12.5 mg/l to 25 mg/l and nor£oxacin MICs of 25 mg/ l to 50 mg/l had single mutations in the gyrA and parC genes. Eight strains with cipro£oxacin MICs of 50 mg/l to 200 mg/l and nor£oxacin MICs of 100 mg/l to 200 mg/l had double mutations in the gyrA gene and single mutations in the parC gene. All the mutations observed in codon 83 of the gyrA gene were C-to-T substitutions, generating an amino acid change of Thr-83CIle. The mutations in codon 87 were G-to-A, G-to-C, and A-to-C substitutions, resulting in amino acid changes of Asp-87CAsn, Asp-87CTyr, and Asp-87CVal, respectively. All the mutations in the codons of the parC gene corresponding to Ser-80 and Glu-84 of the E. coli ParC protein were a G-to-T substitutions, generating Ser80CIle. All the mutations in the codon corresponding to Glu-84 of the E. coli ParC protein were G-toA substitutions, resulting in Glu-84CLys. These alterations observed in GyrA and ParC of C. freundii were analogous to those that were frequently found to be responsible for £uoroquinolone resistance in E. coli and other bacterial species [6,7,12,15^17]. In this study, we found no strains having alterations in
Table 1 Alterations in GyrA and ParC and susceptibilities to cipro£oxacin and nor£oxacin in clinical isolates of C. freundii MIC (mg/l) Amino acid change a a NFLX CPFX GyrA ParC Strain 83 87 80 Type strain 90.025 90.025 Thr(ACC) Asp(GAC) Ser(AGC) ^ ^ 01,11,66 0.1 0.05 ^b 12,58 0.2 0.05 ^ ^ ^ 60,69 0.2 0.1 ^ ^ ^ 04,15 0.78 0.39 ^ ^ ^ 03,07 0.78 0.78 ^ ^ ^ 10,19,65,67 1.56 0.78 ^ ^ ^ 59,68 1.56 1.56 ^ ^ ^ 71,72,73 12.5 6.25 Ile(ATC) ^ ^ 05,06,23,70 25 6.25 Ile(ATC) ^ ^ 02 25 12.5 Ile(ATC) ^ ^ 36 25 12.5 Ile(ATC) ^ Ile(ATC) 34,35 25 25 Ile(ATC) ^ ^ 16,29 50 25 Ile(ATC) ^ Ile(ATC) 18 100 50 Ile(ATC) Tyr(TAC) Ile(ATC) 31,48,51 100 50 Ile(ATC) Tyr(TAC) ^ 55 100 100 Ile(ATC) Tyr(TAC) Ile(ATC) 13,49,50 200 200 Ile(ATC) Val(GTC) Ile(ATC) a NFLX, nor£oxacin; CPFX, cipro£oxacin. b ^, identical to type strain.
FEMSLE 7789 25-10-97
84 Glu(GAA) ^ ^ ^ ^ ^ ^ ^ ^ ^ Lys(AAA) ^ Lys(AAA) ^ ^ Lys(AAA) ^ ^
Y. Nishino et al. / FEMS Microbiology Letters 154 (1997) 409^414
413
Table 2 Antimicrobial susceptibility pro¢les and alterations in GyrA and ParC of pre- and post-treatment
C. freundii
strains isolated from a case
of £uoroquinolone treatment failure in urinary tract infection MICs and alterations
Pre-treatment isolate GU-CF08
Post-treatment isolate GU-CF09
Nor£oxacin
25
100
Cipro£oxacin
12.5
50
O£oxacin
25
50
MIC (mg/l) of :
AM-1155
6.25
Piperacillin
6.25
25 6.25
Cefazolin
3.13
3.13
Cefotaxime
0.78
0.78
Ce¢xime
3.13
3.13
Aztreonam
1.56
1.56
Imipenem
0.2
0.2
Gentamicin
0.39
0.39
Chloramphenicol
0.78
0.78
Tetracycline
3.13
3.13
Alterations in : GyrA
C C
Thr-83
ParC
Ser-80
Ile
C C C
Thr-83
Asp-87
Ile
Ser-80
Ile Asn
Ile
ParC without the simultaneous presence of altera-
tical to each other. These analyses suggested that the
tions in GyrA.
pre- and post-treatment isolates were isogenic. For
The strains having a single or double amino acid
these strains, Table 2 shows the antimicrobial sus-
change in GyrA exhibited signi¢cantly higher-level
ceptibilities and amino acid changes in GyrA and
resistance
ParC. The isolate GU-CF08 exhibited 4-fold higher
to
cipro£oxacin
and
nor£oxacin
than
those without alterations in either GyrA or ParC
MICs
(P
0.01). The six strains with single amino acid
showed MICs of the other agents identical to those
changes in GyrA and ParC were signi¢cantly more
of GU-CF08. In the isolate GU-CF08, the threonine
resistant to cipro£oxacin and nor£oxacin than the
at position 83 was changed into an isoleucine in the
seven strains with a single amino acid change in
GyrA, and the serine at position 80 was substituted
6
GyrA
P
6
alone
(cipro£oxacin,
P
6
0.05 ;
nor£oxacin,
0.01). The eight strains with a double amino
of
£uoroquinolones
than
GU-CF09,
but
C
with an isoleucine in ParC. In the isolate GU-CF09, an alteration of Asp-87
Asn in GyrA was observed
acid change in GyrA and a single amino acid change
in addition to the amino acid changes in GyrA and
in ParC were signi¢cantly more resistant to cipro-
ParC identical to those found in the isolate GU-
£oxacin and nor£oxacin than the six strains with
CF08. The accumulation of amino acid changes in
single
GyrA appeared to contribute to a speci¢c increase in
(P
6
amino
acid
changes
in
GyrA
and
ParC
0.01).
£uoroquinolone resistance in the isolate GU-CF09. In this study, we determined the association of
3.3. Case study of a £uoroquinolone treatment failure in urinary tract infection caused by a quinolone-resistant C. freundii strain
mutations in
gyrA
and
parC
genes with susceptibil-
ities to £uoroquinolones, and reported a case study of a £uoroquinolone treatment failure in an urinary tract infection, accompanied with emergence of a
The electrophoresis pro¢le of the DNAs ampli¢ed
post-treatment isolate with enhanced resistance to
by AP-PCR from the post-treatment isolate GU-
£uoroquinolones. Although we have not proved the
CF09 was identical to that from the pre-treatment
alterations in GyrA and ParC actually cause the re-
isolate GU-CF08. The biochemical characteristics of
sistance phenotype, the ¢ndings of this study do sug-
the pre- and post-treatment isolates also were iden-
gest, in
FEMSLE 7789 25-10-97
C. freundii
as well as in
E. coli
and
N. go-
Y. Nishino et al. / FEMS Microbiology Letters 154 (1997) 409^414
414
norrhoeae,
that DNA gyrase is a primary target of
quinolones, that only a single amino acid change at Thr-83 in GyrA is su¤cient to generate high-level resistance
to
cipro£oxacin
and
nor£oxacin,
and
gyrA and parC in £uoroquinolone-resistant isolates.
regions of
Mol. Microbiol. 14, 371^380. [8] Deguchi, T., Yasuda, M., Asano, M., Tada, K., Iwata, H., Komeda, H., Ezaki, T., Saito, I. and Kawada, Y. (1995) DNA gyrase mutations in quinolone-resistant clinical isolates of
that the accumulation of amino acid changes in
Neisseria gonorrhoeae.
GyrA with the simultaneous presence of alterations
561^563.
in ParC contributes to increment in cipro£oxacin and nor£oxacin resistance [8^10]. To our knowledge, this is the ¢rst report to identify the mutations in the
gyrA
parC
and
genes associated with £uoroquino-
lone resistance in clinical isolates of
C. freundii.
This study should provide useful information for understanding the molecular mechanisms of £uoroquinolone resistance in
C. freundii.
Antimicrob. Agents Chemother. 39,
[9] Georgiou, M., Munoz, R., Roman, F., Canton, R., GomezLus, R., Campos, J. and De la Campa, A.G. (1996) Cipro£oxacin-resistant
Hemophilus in£uenzae
strains possess muta-
tions in analogous positions GyrA and ParC. Antimicrob. Agents Chemother. 40, 1741^1744. [10] Deguchi, T., Yasuda, M., Nakano, M., Ozeki, S., Ezaki, T., Saito, I. and Kawada, Y. (1996) Quinolone-resistant
gonorrhoeae ;
Neisseria
Correlation of alterations in the GyrA subunit
of DNA gyrase and the ParC subunit of topoisomerase IV with antimicrobial susceptibility pro¢les. Antimicrob. Agents Chemother. 40, 1020^1023. [11] Vila, J., Ruiz, J., Goni, P. and Jimenez de Anta, M.T. (1996)
Acknowledgments
parC in quinolone-resistant clinical Escherichia coli. Antimicrob. Agents Chemother.
Detection of mutations in isolates of
40, 491^493.
The authors thank Ms. Kyoko Hirata for technical assistance and laboratory analysis.
[12] Kumagai, Y., Kato, J-I., Hoshino, K., Akasaka, T., Sato, K. and Ikeda, H. (1996) Quinolone-resistant mutants of
chia coli
DNA topoisomerase IV
parC
Escheri-
gene. Antimicrob.
Agents Chemother. 40, 710^714.
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FEMSLE 7789 25-10-97