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Mitogenic effects of beryllium and zirconium salts on mouse splenocytes in vitro
Toxicology
Letters,
30 (1986) 89-95
89
Elsevier
TOXLett.
1530
MITOGENIC EFFECTS OF BERYLLIUM MOUSE SPLENOCYTES IN VITRO
AND ZIRCONIUM
(Beryllium; zirconium; mouse splenocytes; lymphocytes; ROGER MRC
J. PRICE Toxicology
Surrey,
and DAVID
SALTS ON
mitogenesis)
N. SKILLETER
Unit, Medical
Research
Council
Laboratories,
Woodmansterne
Road,
Carshalton,
SM.5 4EF (U.K.)
(Received
October
8th,
(Revision
received
and accepted
1985) November
28th,
1985)
(Zr) salts,
BeSO
SUMMARY The beryllium dependent incorporation 100-200
into lymphocyte
to assist
results indicate augment
of mouse
pM) was greater
low concentrations found
(Be) and zirconium
stimulation
tion of delayed
DNA, although
subsequent that at defined
(concanavalin
concentrations
responsiveness
hypersensitivity
as measured response
each exerted by an increase induced
range of Zr(SO&
concentrations
A; ConA)-mediated
a concentrationin [3H]thymidine
by Zr(SO&
(2-3 fold at l-5 FM). Preincubation
(< 1 PM) or a broad lectin
and Zr(SO&,
the maximal
than that by BeSO
of BeSO
the functional
spleen cell proliferation
and production
lymphocyte
proliferation.
granulomas
The
mitogens
cells, which may help explain the characteristic of immunological
with
(2-100 PM) was also
Be and Zr salts can both act as lymphocyte
of immune
(4-5 fold at
of splenocytes
by these metals
and
inducin viva.
INTRODUCTION
The metals Be and Zr have important applications in the nuclear, aerospace and metal alloy industries as well as other specialised uses [1,2]. A characteristic of human exposure to these metals and some of their compounds is the development in many individuals of cell (T-lymphocyte)-mediated delayed skin hypersensitivity followed by the appearance of immunological granulomas [3,4]. These granulomas are described by the presence of giant and epithelioid cells of mononuclear phagocyte origin associated with lymphocyte infiltration and contrast with the granulomas produced by metals such as aluminium which contain mainly phagocytosing macrophages and have been described as non-immunological [5]. Abbreviations:
0378-4274/86/$
ConA,
concanavalin
03.50 0 Elsevier
A; IL, interleukin;
Science
Publishers
TCA,
trichloroacetic
B.V. (Biomedical
acid.
Division)
90
Although the in vivo immunotoxicology of Be and Zr has been extensively studied in experimental animals [5,6], relatively little is known about the effects these metals have on immune cells in vitro. Cells isolated from spleen are known to comprise both lymphocyte and accessory (adherent macrophage type) populations and thus provide a useful in vitro system to monitor certain immune cell properties particularly mitogenic responses 171. In the present study, using the incorporation of [3H]thymidine into cultured mouse spleen lymphocyte DNA as a measure of cell proliferation, we have examined both the direct mitogenic effects of Be and Zr salts and the consequences of treatment of splenocytes with the metal salts on their subsequent response to lectin mitogens. The results indicate that Be and Zr salts stimulate lymphocyte proliferation and augment subsequent lectin-mediated mitogenesis, but that these reponses are strongly concentration-dependent. MATERIALS
AND METHODS
Materials Metal salts of analytical grade were obtained from Aldrich Chemical Co. Ltd., Gillingham, Dorset (U.K.) and aqueous solutions (1 mM) were freshly prepared before use and maintained at pH 5.0 to avoid formation of colloidal precipitates. All metal ion solutions and ConA (Sigma Chemical Co., Poole, Dorset, U.K.) were filtered through a 0.22 FM MiIlipore filter prior to addition to the culture media. The lymphocyte culture medium (RPM1 1640) was purchased from Gibco-Europe, Paisley, Scotland; foetal calf serum from Sera Lab., Crawley Down, Sussex; phosphate-buffered saline (Dulbecco A) from Oxoid Ltd., Basingstoke, Hampshire, and flat-bottomed 3.5ml capacity Linbro multi-well culture plates from Flow Laboratories, Irvine, Scotland. [3H]Thymidine was obtained from Amersham International, Bucks (U.K.). Preparation of spleen cells Spleens from COz-killed adult male MFI mice (20-25 g), were gently handhomogenized in 10 ml RPM1 1640 and filtered through a 250~PM mesh nylon gauze. The filtrate was centrifuged (200 x g, 1 min) to remove debris and the supernatant mixed with 2 ~01s. 0.87% NH&l to lyse red blood cells. The splenocytes were centrifuged (350 x g, 10 min) and washed in RPM1 1640, and finally filtered through a lOO-PM nylon gauze. The cell yield was approx. 45 x lo6 lymphocytes per mouse spleen and contained approx. O. l-0.2% adherent cells. Cell viability was measured throughout the study by trypan blue dye exclusion and estimated to be 85-90% in freshly isolated cells. Lymphocyte incubations Splenocytes (2.5 x lo6 cells) were incubated in the presence or absence of metal
91
ion additions in 1 ml RPM1 1640 medium containing 5% heat-inactivated foetal calf serum maintained in culture plates at 37°C pH 7.3 in a humidified atmosphere of 95% air 5% CO2. When used ConA was included in the medium at an optimal concentration of 2 pg/ml, cell proliferation was measured after the indicated treatments by a 2-h pulse-labelled [3H]thymidine (0.1 &i) incorporation into lymphocyte DNA. The aspirated well contents were sequentially centrifuged (300 x g, 10 min) and washed with 1 ml RPM1 1640 and 3 ml phosphate-buffered saline, followed by precipitation overnight at 0°C in 5% TCA. The centrifuged (2500 x g, 10 min) tissue pellet was dissolved in 0.5 ml 1 M NaOH overnight mixed with 0.5 ml distilled water, 100 ~1glacial acetic acid and 10 ml Beckman MP Scintillant prior to measurement of 3H-radioactivity in a Packard Tri-Carb Model 460 scintillation counter. RESULTS AND DISCUSSION
Fig. 1 shows that after an optimum incubation period of 3 days Zr(SO& was a more effective mitogen to mouse splenocytes than BeSOd. Furthermore, stimulation of [3H]thymidine incorporation into lymphocyte DNA was produced by only a narrow range of BeSO concentrations (l-5 PM) whereas maximal effects of Zr(SO& were observed over a much broader and higher concentration range (20-200 PM). 10-
0
I 20
5 Metal
I I I loo 200 300 400
salt concentration
(@II
Fig. 1. Comparison of the stimulation of mouse spleen lymphocyte DNA synthesis by beryllium and zirconium. Mouse splenocytes (2.5 x lo6 cells) were incubated in the presence of various concentrations (abscissa) of either BeSO (0), Zr(SO)d (0) or Ah(S04)3 (A) for 3 days prior to measurement of pulselabelled
[3H]thymidine
5 determinations.
incorporation
(2 h) into lymphocyte
DNA. Values (ordinate)
are means
+ SD of
92
No incorporation of radiolabel was detected in the presence of 10 mM hydroxyurea, demonstrating that the metal salt stimulation was due to replicative DNA synthesis and not unscheduled DNA repair [8,9]. The metal ions Hg’ + and Zn’ ’ have been shown to induce lymphocyte proliferation in vitro with optima at approx. 10 PM and 100 pM, respectively, possibly by direct action of the metal ions on T-cells HO-121 and we have demonstrated previously Be2 + binding to lymphocytes [22]. Both Be and Zr salts readily form hydroxides at physiological pH and thus differences in the dose-response of lymphocyte replication to these metal salts may simply be a reflection of the proportions and availablility of free metal ions. In this respect it would be of value to know the differential hydroxide precipitation characteristics of BeS04 and Zr(SO& in the culture medium but the detailed analyses required for this estimation have yet to be carried out. The decrease in [3H]thymidine incorporation induced by metal salt concentrations above 5 pM BeSO or 200 PM Zr(S04)2 may have been associated with some cytotoxic effects since the presence of 50-100 FM BeSO or 200-400 pM Zr(SO& was shown to cause a 25% and 15% loss of cell viability respectively. However, a more probable explanation might be that of an opposing effect of the inhibition of cell division since it is known that, at least in non lymphoid cells, intracellular access of a number of metal ions including Be’+ can block DNA synthesis [24,25]. Facilitation of T-lymphocyte activation by lectin mitogens requires the presence of accessory cells [ 13,141 which were known to be present in the splenocyte preparations. Pretreatment of splenocytes with compounds followed by lectin stimulation can thus be used to monitor affects of such materials on the normal mitogenic response of lymphoid cells [7]. We have used this approach to examine the action of optimal and suboptimal mitogenic concentrations of BeSO and Zr(SO& on the subsequent response of splenocytes to ConA. A characteristic of our in vitro test system was that a 20-h preincubation of cells in the absence of lectin resulted in an 80% decrease in the ConA-stimulated [3H]thymidine incorporation into lymphocyte DNA. Our earlier studies had established that this was due to loss of the accessory cells or their activation factors from the culture since ConA responsiveness could be restored by subsequent addition of macrophages [23]. However, Table I shows that pretreatment with appropriate concentrations of BeSO or Zr(SO& for 20 h substantially maintained the proliferative response. This was most marked in the case of Zr(SO4)z for which a 40-60% retention of lymphocyte responsiveness to ConA was achieved over a broad range of concentrations (20-100 yM) and thus the effect appeared to be independent of the Zr(SO& concentrations already shown to cause direct mitogenesis (cf. Fig. 1). In contrast only pretreatment of splenocytes with a normally nonmitogenic concentration of BeSO (viz. 0.2 FM) resulted in a significant retention of the response to ConA, concentrations above 1 pM BeSO being strongly inhibitory (Table I). A similar marked loss of lymphocyte responsiveness to mitogens in vitro has been
93
TABLE
I
EFFECT
OF PREINCUBATION
CONIUM Mouse
ON SUBSEQUENT
splenocytes
OF MOUSE RESPONSE
(2.5 x lo6 cells) were incubated
serum at 37°C for 20 h under the preincubation in the presence
of 2 a&/ml ConA
into lymphocyte Preincubation
SPLENOCYTES
TO CONCANAVALIN
DNA.
and measurement
Values are means
conditions
in RPM1
conditions
WITH
1640 medium
indicated
of pulse-labelled
BERYLLIUM
AND
ZIR-
A containing
prior to a further 13H]thymidine
5% foetal calf 3 days incubation
incorporation
(2 h)
k SD of 5 determinations.
Proliferation
response
incorporation
(dpm)
to ConA
[jH]thymidine
Control (no preincubation)a
76 286 f
No additions
14 929 + 1797
BeSO
0.2 gM
29 874 + 3988
1.0 FM
13 326 i
5.0 PM Zr(S0)4
2 CM
790 +-
8550
1244 278
35 257 + 3331
20 PM
41 966 * 5210
100 NM
47 484 r 7898
a Incubation
in the presence
of ConA
(2 pg/ml)
for 3 days without
any preincubation
treatment.
observed following pretreatment of splenocytes with silica or carbonyl iron and shown to result from adherent cell destruction [7]. Mononuclear phagocytes are known to be extremely sensitive to the cytotoxicity of several Be compounds [15-171 and consequently the loss of BeSO augmented ConA mitogenesis above 1 FM BeSO might also have been caused by elimination of the adherent cell population. We were able to substantiate this conclusion from examination of the culture dishes by light microscopy which revealed a severe loss of the adherent cells. In contrast Zr(SO& caused little loss of adherent cells which suggests that it was relatively noncytotoxic to macrophages, a conclusion supported by the evidence that this is known to be the case for Zr(OH)d [lS], a major product generated from Zr(SO& in the culture medium. At present the mechanism by which pretreatment with Zr(SO&, or low concentrations of BeS04, maintained subsequent ConA-induced mitogenesis is not clear. However, Zr and Be may enhance the functional responsiveness of immune cells through stimulation of IL1 secretion by the macrophage population with resultant lymphocyte (T-cell) proIiferation via IL2 production 1191. There is some experimental evidence that BeSO can activate IL1 release [20] and such a response might also play a role in the direct mitogenic effects of the metal salt since the release of IL1 and other lymphocyte growth factors from damaged macrophages and lymphocytes could contribute to the proliferative stimulus [19,21]. It is hoped that future studies might provide data to substantiate these suggestions. In the course of our study we also examined the effects of aluminium salts on mouse splenocytes since in vivo these compounds have been considered to produce
94
only nonimmunological granulomas [5]. We were unable to demonstrate any mitogenic properties of Al2 (SO& (Fig. 1) and pretreatment of spleen cells with the metal salt (l-50 PM) eliminated ConA-induced lymphocyte proliferation. Al salts have similar physicochemical properties to those of Be and Zr in that they too readily form hydroxides at physiological pH; furthermore, previous studies have shown that colloidal Al(OH)3 is highly cytotoxic to macrophages [18]. A probable interpretation of the present findings therefore is that the induction of delayed hypersensitivity and production of the distinctive immunological granulomas by certain Zr and Be compounds in vivo may in part be related to their dose-dependent properties of directly stimulating and, through interaction with macrophages, indirectly augmenting lymphocyte proliferative responses to other agents.
REFERENCES 1 L.B. Tepper, York, 2 P.B.
Beryllium,
in H.A.
Waldron
(Ed.),
Metals in the Environment,
A:ademic
Press,
New
1980, Ch. 2, pp. 25-60. Hammond
Cassarett
and
R.P.
Beliles,
and Doull’s Toxicology,
Metals,
in J. Doull,
C.D.
Klassen
the Basic Science of Poisons,
and
M.O.
Amdur
2nd ed., Macmillan,
(Eds.),
London,
1980,
Ch. 17, pp. 409-467. 3 W.B. Shelley and H.J. in man, Nature, 4 M.M.
Hurley,
Black and W.L.
granulomas,
Epstein,
Am. J. Pathol.,
5 J.L. Turk and D. Parker, bard 6 A.L.
and D.V. Parke
Formation
Immunological
(Eds.),
Immunotoxicology,
7 U. Persson,
W.G.
9 A.D. Mitchell, Mutation
Res.,
10 H. Kirschner
Press,
E. Moller, Immunol.
Flamm
formation
epithelioid
cell
Academic
and N.J.
in G.G.
New York,
in G.G. Gibson,
New York,
Gibson,
R. Hub-
1983, pp. 251-259.
R. Hubbard
and D.V. Parke
1983, pp. 261-282.
G. Moller and C.I.E.
Bernheim,
Smith,
Role of adherent
The value of hydroxyurea
Interact.,
cells in B
test, A report
in assessing
repair
syn-
5 (1972) 327-339.
M.L. Meltz, E. Robinson,
DNA synthesis
formation, Press,
Rev., 40 (1978) 78-101.
cells, Chem.-Biol.
D.A. Casciano,
Unscheduled
giant cells in organised
aspects of granuloma of beryllium,
Academic
activation,
thesis of DNA in HeLa Halle,
for an allergic basis for granuloma
of multinucleate
Immunotoxicology,
L. Hammerstrom,
and T lymphocyte Brandt,
evidence
74 (1974) 263-274.
Reeves, The immunotoxicology
(Eds.),
8 W.N.
Experimental
180 (1957) 1060-1061.
R.H.C.
San, G.M. Williams
of the US Protection
Agency
and E.S. van
gene-tox
program,
123 (1983) 363-410.
and H. Ruhl, Stimulation
of human
peripheral
lymphocytes
by Zn’+ in vitro, Exp. Cell.
Res., 61 (1970) 229-230. 1 I N.A. Berger and A.M. Skinner, J. Cell Biol., 61 (1974) 45-55. 12 D.A. Hart,
Effect of zinc chloride
ment of lipopolysaccharide 13 D.L.
Rosenstreich,
phocyte activation 14 D.L. Rosenstreich the activation 15 P. Camner, different
Characterisation
J.J.
Farrow
lymphoid
of lymphocytes,
and S. Dougherty,
transformation
cells: mitogenicity Infect.
Absolute
Immun., macrophage
by mitogens J. Immunol., 116 (1976) 131-139. and S.B. Migel, The participation of macrophages
of T lymphocytes M. Lundborg
metals,
on hamster
stimulation
of lymphocyte
Arch.
by mitogens,
and P.A. Hellstrom, Environ.
Health,
lmmunol. Alveolar
induced
by zinc ions,
and differential
enhance-
19 (1978) 457-461. dependence
and macrophage
of T lymcell lines in
Rev., 40 (1978) 102-135. macrophages
29 (1974) 21 l-213.
and 5 pM particles
coated with
95 16 K.Y. Kang and J. Salvaggio, Effect of asbestos and beryllium compounds on the alveolar macrophage, Med. J. Osaka Univ., 27 (1976) 47-58. 17 D.N. Skilleter and R.J. Price, Effects of beryllium on rat liver Kupffer cells in culture, Toxicol. Appl. Pharmacol., 59 (1981) 279-286. 18 P. Badenoch-Jones, J.L. Turk and D. Parker, The effects of some aluminium and zirconium compounds on guinea-pig peritoneal macrophages and skin fibrobiasts, J. Pathoi., 124 (1978) 51-62. 19 A.L. Maize1 and L.B. Lachman, Biology of disease. Control of human lymphocyte proliferation by soluble factors, Lab. Invest., 50 (1984) 369-377. 20 E.R. Unanue, J.M. Kieiy and J. Caideron, The modulation of lymphocyte functions by molecules secreted by macrophages, II. Conditions leading to increased secretion, J. Exp. Med., 144 (1976) 155-166. 21 J.G. Hail, Studies on the adjuvant action of beryllium. I Effects on individual lymph nodes, Immunology, 53 (1984) 105-113. 22 D.N. Skifleter and R.J. Price, Lymphocyte beryllium binding: Relationship to development of delayed beryllium hypersensitivity, int. Arch. Allergy Appl. lmmun., 73 (1984) 181-183. 23 R.J Price and D.N. Skiiieter, Stimuiatory and cytotoxic effects of beryllium on proliferation of mouse spleen lymphocytes in vitro, Arch. Toxicol., 56 (1985) 207-21 I. 24 M. Costa, 0. Cantoni, M. de Mars and D.E. Swartzendruber, Toxic metals produce an S-phase specific cell cycle block, Res. Commun. Chem. Pathol. Pharmacol., 38 (1982) 405-419. 25 D.N. Skilieter, R.J. Price and R.F. Legg, Specific Gr-S phase ceil cycle block by beryllium as deomonstrated by cytofluorometric analysis, Biochem. J., 216 (1983) 773-776.
Letters,
30 (1986) 89-95
89
Elsevier
TOXLett.
1530
MITOGENIC EFFECTS OF BERYLLIUM MOUSE SPLENOCYTES IN VITRO
AND ZIRCONIUM
(Beryllium; zirconium; mouse splenocytes; lymphocytes; ROGER MRC
J. PRICE Toxicology
Surrey,
and DAVID
SALTS ON
mitogenesis)
N. SKILLETER
Unit, Medical
Research
Council
Laboratories,
Woodmansterne
Road,
Carshalton,
SM.5 4EF (U.K.)
(Received
October
8th,
(Revision
received
and accepted
1985) November
28th,
1985)
(Zr) salts,
BeSO
SUMMARY The beryllium dependent incorporation 100-200
into lymphocyte
to assist
results indicate augment
of mouse
pM) was greater
low concentrations found
(Be) and zirconium
stimulation
tion of delayed
DNA, although
subsequent that at defined
(concanavalin
concentrations
responsiveness
hypersensitivity
as measured response
each exerted by an increase induced
range of Zr(SO&
concentrations
A; ConA)-mediated
a concentrationin [3H]thymidine
by Zr(SO&
(2-3 fold at l-5 FM). Preincubation
(< 1 PM) or a broad lectin
and Zr(SO&,
the maximal
than that by BeSO
of BeSO
the functional
spleen cell proliferation
and production
lymphocyte
proliferation.
granulomas
The
mitogens
cells, which may help explain the characteristic of immunological
with
(2-100 PM) was also
Be and Zr salts can both act as lymphocyte
of immune
(4-5 fold at
of splenocytes
by these metals
and
inducin viva.
INTRODUCTION
The metals Be and Zr have important applications in the nuclear, aerospace and metal alloy industries as well as other specialised uses [1,2]. A characteristic of human exposure to these metals and some of their compounds is the development in many individuals of cell (T-lymphocyte)-mediated delayed skin hypersensitivity followed by the appearance of immunological granulomas [3,4]. These granulomas are described by the presence of giant and epithelioid cells of mononuclear phagocyte origin associated with lymphocyte infiltration and contrast with the granulomas produced by metals such as aluminium which contain mainly phagocytosing macrophages and have been described as non-immunological [5]. Abbreviations:
0378-4274/86/$
ConA,
concanavalin
03.50 0 Elsevier
A; IL, interleukin;
Science
Publishers
TCA,
trichloroacetic
B.V. (Biomedical
acid.
Division)
90
Although the in vivo immunotoxicology of Be and Zr has been extensively studied in experimental animals [5,6], relatively little is known about the effects these metals have on immune cells in vitro. Cells isolated from spleen are known to comprise both lymphocyte and accessory (adherent macrophage type) populations and thus provide a useful in vitro system to monitor certain immune cell properties particularly mitogenic responses 171. In the present study, using the incorporation of [3H]thymidine into cultured mouse spleen lymphocyte DNA as a measure of cell proliferation, we have examined both the direct mitogenic effects of Be and Zr salts and the consequences of treatment of splenocytes with the metal salts on their subsequent response to lectin mitogens. The results indicate that Be and Zr salts stimulate lymphocyte proliferation and augment subsequent lectin-mediated mitogenesis, but that these reponses are strongly concentration-dependent. MATERIALS
AND METHODS
Materials Metal salts of analytical grade were obtained from Aldrich Chemical Co. Ltd., Gillingham, Dorset (U.K.) and aqueous solutions (1 mM) were freshly prepared before use and maintained at pH 5.0 to avoid formation of colloidal precipitates. All metal ion solutions and ConA (Sigma Chemical Co., Poole, Dorset, U.K.) were filtered through a 0.22 FM MiIlipore filter prior to addition to the culture media. The lymphocyte culture medium (RPM1 1640) was purchased from Gibco-Europe, Paisley, Scotland; foetal calf serum from Sera Lab., Crawley Down, Sussex; phosphate-buffered saline (Dulbecco A) from Oxoid Ltd., Basingstoke, Hampshire, and flat-bottomed 3.5ml capacity Linbro multi-well culture plates from Flow Laboratories, Irvine, Scotland. [3H]Thymidine was obtained from Amersham International, Bucks (U.K.). Preparation of spleen cells Spleens from COz-killed adult male MFI mice (20-25 g), were gently handhomogenized in 10 ml RPM1 1640 and filtered through a 250~PM mesh nylon gauze. The filtrate was centrifuged (200 x g, 1 min) to remove debris and the supernatant mixed with 2 ~01s. 0.87% NH&l to lyse red blood cells. The splenocytes were centrifuged (350 x g, 10 min) and washed in RPM1 1640, and finally filtered through a lOO-PM nylon gauze. The cell yield was approx. 45 x lo6 lymphocytes per mouse spleen and contained approx. O. l-0.2% adherent cells. Cell viability was measured throughout the study by trypan blue dye exclusion and estimated to be 85-90% in freshly isolated cells. Lymphocyte incubations Splenocytes (2.5 x lo6 cells) were incubated in the presence or absence of metal
91
ion additions in 1 ml RPM1 1640 medium containing 5% heat-inactivated foetal calf serum maintained in culture plates at 37°C pH 7.3 in a humidified atmosphere of 95% air 5% CO2. When used ConA was included in the medium at an optimal concentration of 2 pg/ml, cell proliferation was measured after the indicated treatments by a 2-h pulse-labelled [3H]thymidine (0.1 &i) incorporation into lymphocyte DNA. The aspirated well contents were sequentially centrifuged (300 x g, 10 min) and washed with 1 ml RPM1 1640 and 3 ml phosphate-buffered saline, followed by precipitation overnight at 0°C in 5% TCA. The centrifuged (2500 x g, 10 min) tissue pellet was dissolved in 0.5 ml 1 M NaOH overnight mixed with 0.5 ml distilled water, 100 ~1glacial acetic acid and 10 ml Beckman MP Scintillant prior to measurement of 3H-radioactivity in a Packard Tri-Carb Model 460 scintillation counter. RESULTS AND DISCUSSION
Fig. 1 shows that after an optimum incubation period of 3 days Zr(SO& was a more effective mitogen to mouse splenocytes than BeSOd. Furthermore, stimulation of [3H]thymidine incorporation into lymphocyte DNA was produced by only a narrow range of BeSO concentrations (l-5 PM) whereas maximal effects of Zr(SO& were observed over a much broader and higher concentration range (20-200 PM). 10-
0
I 20
5 Metal
I I I loo 200 300 400
salt concentration
(@II
Fig. 1. Comparison of the stimulation of mouse spleen lymphocyte DNA synthesis by beryllium and zirconium. Mouse splenocytes (2.5 x lo6 cells) were incubated in the presence of various concentrations (abscissa) of either BeSO (0), Zr(SO)d (0) or Ah(S04)3 (A) for 3 days prior to measurement of pulselabelled
[3H]thymidine
5 determinations.
incorporation
(2 h) into lymphocyte
DNA. Values (ordinate)
are means
+ SD of
92
No incorporation of radiolabel was detected in the presence of 10 mM hydroxyurea, demonstrating that the metal salt stimulation was due to replicative DNA synthesis and not unscheduled DNA repair [8,9]. The metal ions Hg’ + and Zn’ ’ have been shown to induce lymphocyte proliferation in vitro with optima at approx. 10 PM and 100 pM, respectively, possibly by direct action of the metal ions on T-cells HO-121 and we have demonstrated previously Be2 + binding to lymphocytes [22]. Both Be and Zr salts readily form hydroxides at physiological pH and thus differences in the dose-response of lymphocyte replication to these metal salts may simply be a reflection of the proportions and availablility of free metal ions. In this respect it would be of value to know the differential hydroxide precipitation characteristics of BeS04 and Zr(SO& in the culture medium but the detailed analyses required for this estimation have yet to be carried out. The decrease in [3H]thymidine incorporation induced by metal salt concentrations above 5 pM BeSO or 200 PM Zr(S04)2 may have been associated with some cytotoxic effects since the presence of 50-100 FM BeSO or 200-400 pM Zr(SO& was shown to cause a 25% and 15% loss of cell viability respectively. However, a more probable explanation might be that of an opposing effect of the inhibition of cell division since it is known that, at least in non lymphoid cells, intracellular access of a number of metal ions including Be’+ can block DNA synthesis [24,25]. Facilitation of T-lymphocyte activation by lectin mitogens requires the presence of accessory cells [ 13,141 which were known to be present in the splenocyte preparations. Pretreatment of splenocytes with compounds followed by lectin stimulation can thus be used to monitor affects of such materials on the normal mitogenic response of lymphoid cells [7]. We have used this approach to examine the action of optimal and suboptimal mitogenic concentrations of BeSO and Zr(SO& on the subsequent response of splenocytes to ConA. A characteristic of our in vitro test system was that a 20-h preincubation of cells in the absence of lectin resulted in an 80% decrease in the ConA-stimulated [3H]thymidine incorporation into lymphocyte DNA. Our earlier studies had established that this was due to loss of the accessory cells or their activation factors from the culture since ConA responsiveness could be restored by subsequent addition of macrophages [23]. However, Table I shows that pretreatment with appropriate concentrations of BeSO or Zr(SO& for 20 h substantially maintained the proliferative response. This was most marked in the case of Zr(SO4)z for which a 40-60% retention of lymphocyte responsiveness to ConA was achieved over a broad range of concentrations (20-100 yM) and thus the effect appeared to be independent of the Zr(SO& concentrations already shown to cause direct mitogenesis (cf. Fig. 1). In contrast only pretreatment of splenocytes with a normally nonmitogenic concentration of BeSO (viz. 0.2 FM) resulted in a significant retention of the response to ConA, concentrations above 1 pM BeSO being strongly inhibitory (Table I). A similar marked loss of lymphocyte responsiveness to mitogens in vitro has been
93
TABLE
I
EFFECT
OF PREINCUBATION
CONIUM Mouse
ON SUBSEQUENT
splenocytes
OF MOUSE RESPONSE
(2.5 x lo6 cells) were incubated
serum at 37°C for 20 h under the preincubation in the presence
of 2 a&/ml ConA
into lymphocyte Preincubation
SPLENOCYTES
TO CONCANAVALIN
DNA.
and measurement
Values are means
conditions
in RPM1
conditions
WITH
1640 medium
indicated
of pulse-labelled
BERYLLIUM
AND
ZIR-
A containing
prior to a further 13H]thymidine
5% foetal calf 3 days incubation
incorporation
(2 h)
k SD of 5 determinations.
Proliferation
response
incorporation
(dpm)
to ConA
[jH]thymidine
Control (no preincubation)a
76 286 f
No additions
14 929 + 1797
BeSO
0.2 gM
29 874 + 3988
1.0 FM
13 326 i
5.0 PM Zr(S0)4
2 CM
790 +-
8550
1244 278
35 257 + 3331
20 PM
41 966 * 5210
100 NM
47 484 r 7898
a Incubation
in the presence
of ConA
(2 pg/ml)
for 3 days without
any preincubation
treatment.
observed following pretreatment of splenocytes with silica or carbonyl iron and shown to result from adherent cell destruction [7]. Mononuclear phagocytes are known to be extremely sensitive to the cytotoxicity of several Be compounds [15-171 and consequently the loss of BeSO augmented ConA mitogenesis above 1 FM BeSO might also have been caused by elimination of the adherent cell population. We were able to substantiate this conclusion from examination of the culture dishes by light microscopy which revealed a severe loss of the adherent cells. In contrast Zr(SO& caused little loss of adherent cells which suggests that it was relatively noncytotoxic to macrophages, a conclusion supported by the evidence that this is known to be the case for Zr(OH)d [lS], a major product generated from Zr(SO& in the culture medium. At present the mechanism by which pretreatment with Zr(SO&, or low concentrations of BeS04, maintained subsequent ConA-induced mitogenesis is not clear. However, Zr and Be may enhance the functional responsiveness of immune cells through stimulation of IL1 secretion by the macrophage population with resultant lymphocyte (T-cell) proIiferation via IL2 production 1191. There is some experimental evidence that BeSO can activate IL1 release [20] and such a response might also play a role in the direct mitogenic effects of the metal salt since the release of IL1 and other lymphocyte growth factors from damaged macrophages and lymphocytes could contribute to the proliferative stimulus [19,21]. It is hoped that future studies might provide data to substantiate these suggestions. In the course of our study we also examined the effects of aluminium salts on mouse splenocytes since in vivo these compounds have been considered to produce
94
only nonimmunological granulomas [5]. We were unable to demonstrate any mitogenic properties of Al2 (SO& (Fig. 1) and pretreatment of spleen cells with the metal salt (l-50 PM) eliminated ConA-induced lymphocyte proliferation. Al salts have similar physicochemical properties to those of Be and Zr in that they too readily form hydroxides at physiological pH; furthermore, previous studies have shown that colloidal Al(OH)3 is highly cytotoxic to macrophages [18]. A probable interpretation of the present findings therefore is that the induction of delayed hypersensitivity and production of the distinctive immunological granulomas by certain Zr and Be compounds in vivo may in part be related to their dose-dependent properties of directly stimulating and, through interaction with macrophages, indirectly augmenting lymphocyte proliferative responses to other agents.
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