METABOLIC-INHIBITORS DISTINGUISH CYTOLYTIC ACTIVITY OF CD4 AND CD8 CLONES

被引：45

作者：

STRACK, P

MARTIN, C

SAITO, S

DEKRUYFF, RH

JU, ST

机构：

[1] BOSTON UNIV,SCH MED,CTR ARTHRITIS,K510,BOSTON,MA 02118

[2] HARVARD UNIV,SCH MED,DEPT PATHOL,BOSTON,MA 02115

[3] CHILDRENS HOSP,DEPT PEDIAT,PALO ALTO,CA

来源：

EUROPEAN JOURNAL OF IMMUNOLOGY | 1990年 / 20卷 / 01期

关键词：

D O I：

10.1002/eji.1830200126

中图分类号：

R392 [医学免疫学]; Q939.91 [免疫学];

学科分类号：

100102 ;

摘要：

The effect of various metabolic inhibitors on the expression of cytolytic activity of CD4 (TH1) and CD8 (CTL) clones was studied. The cytolytic activity of CD4 clones, but not CD8 clones, was sensitive to the RNA synthesis inhibitor actinomycin D and the protein synthesis inhibitor cycloheximide. Conversely, cholera toxin (CT) inhibited cytolytic activity of CD8, but not CD4 clones. Both mitomycin C, a DNA synthesis inhibitor, and cyclosporin A (CsA) failed to inhibit the cytolytic activity of either CD4 or CD8 clones. Although pretreatment with CsA or CT did not inhibit the cytolytic activity of CD4 clones, lymphokine (interleukin 2, IL 2, interferon‐γ, IFN‐γ, and tumor necrosis factor, TNF) production was strongly inhibited. Similarly, pretreatment of a CD8 clone with actinomycin D or CsA inhibited lymphokine production without affecting cytolytic activity. The production of mRNA for TNF and IFN‐γ by concanavalin A‐activated CD4 clones was also inhibited by CsA and CT. Moreover, perforin‐specific mRNA was not detected in activated CD4 clones. Collectively, these observations demonstrated that de novo synthesis of RNA and protein is required for expression of cytolytic activity of CD4 clones, yet production of TNF, INF‐γ, IL 2 and perforin is not involved. In contrast, the cytolytic machinery of CD8 clones is present prior to activation and is quickly expressed following activation even when de novo synthesis of RNA, protein and lymphokines is blocked. Copyright © 1990 WILEY‐VCH Verlag GmbH & Co. KGaA, Weinheim

引用

页码：179 / 184

页数：6

共 39 条

[1] CYCLOSPORIN-A MEDIATES IMMUNOSUPPRESSION OF PRIMARY CYTO-TOXIC T-CELL RESPONSES BY IMPAIRING THE RELEASE OF INTERLEUKIN-1 AND INTERLEUKIN-2
BUNJES, D
HARDT, C
ROLLINGHOFF, M
WAGNER, H
[J]. EUROPEAN JOURNAL OF IMMUNOLOGY, 1981, 11 (08) : 657 - 661
[2] IDENTIFICATION OF A COMMON NUCLEOTIDE-SEQUENCE IN THE 3'-UNTRANSLATED REGION OF MESSENGER-RNA MOLECULES SPECIFYING INFLAMMATORY MEDIATORS
CAPUT, D
BEUTLER, B
HARTOG, K
THAYER, R
BROWNSHIMER, S
CERAMI, A
[J]. PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1986, 83 (06) : 1670 - 1674
[3] CHANG JCC, 1986, J IMMUNOL, V136, P2826
[4] CHANG TW, 1980, J IMMUNOL, V124, P1028
[5] ANALYSIS OF T-CELL RESPONSES TO POLY-L(GLULYS) AT THE CLONAL LEVEL .1. PRESENCE OF RESPONSIVE CLONES IN NONRESPONDER MICE
DEKRUYFF, RH
JU, ST
LANING, J
DORF, ME
[J]. EUROPEAN JOURNAL OF IMMUNOLOGY, 1987, 17 (08) : 1115 - 1120
[6] DOHERTY PC, 1976, TRANSPLANT REV, V29, P89
[7] INDUCTION OF INTERLEUKIN-2 MESSENGER-RNA INHIBITED BY CYCLOSPORIN-A
ELLIOTT, JF
LIN, YA
MIZEL, SB
BLEACKLEY, RC
HARNISH, DG
PAETKAU, V
[J]. SCIENCE, 1984, 226 (4681) : 1439 - 1441
[8] ACTIVATION OF THE HUMAN INTERFERON-BETA GENE REQUIRES AN INTERFERON-INDUCIBLE FACTOR
ENOCH, T
ZINN, K
MANIATIS, T
[J]. MOLECULAR AND CELLULAR BIOLOGY, 1986, 6 (03) : 801 - 810
[9] PERFORIN IS PRESENT ONLY IN NORMAL ACTIVATED LYT2+ LYMPHOCYTES-T AND NOT IN L3T4+ CELLS, BUT THE SERINE PROTEASE GRANZYME-A IS MADE BY BOTH SUBSETS
GARCIASANZ, JA
PLAETINCK, G
VELOTTI, F
MASSON, D
TSCHOPP, J
MACDONALD, HR
NABHOLZ, M
[J]. EMBO JOURNAL, 1987, 6 (04) : 933 - 938
[10] TRANSMEMBRANE SIGNALING BY THE T-CELL ANTIGEN RECEPTOR - PERTURBATION OF THE T3-ANTIGEN RECEPTOR COMPLEX GENERATES INOSITOL PHOSPHATES AND RELEASES CALCIUM-IONS FROM INTRACELLULAR STORES
IMBODEN, JB
STOBO, JD
[J]. JOURNAL OF EXPERIMENTAL MEDICINE, 1985, 161 (03) : 446 - 456

← 1 2 3 4 →