BIOCHEMICAL-EVIDENCE OF THE PHYSICAL ASSOCIATION OF THE MAJORITY OF CD3 DELTA-CHAINS WITH THE ACCESSORY CORECEPTOR MOLECULES CD4 AND CD8 ON NONACTIVATED LYMPHOCYTES-T
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SUZUKI, S
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MAX PLANCK INST IMMUNBIOL,W-7800 FREIBURG,GERMANYMAX PLANCK INST IMMUNBIOL,W-7800 FREIBURG,GERMANY
SUZUKI, S
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KUPSCH, J
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MAX PLANCK INST IMMUNBIOL,W-7800 FREIBURG,GERMANYMAX PLANCK INST IMMUNBIOL,W-7800 FREIBURG,GERMANY
KUPSCH, J
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EICHMANN, K
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MAX PLANCK INST IMMUNBIOL,W-7800 FREIBURG,GERMANYMAX PLANCK INST IMMUNBIOL,W-7800 FREIBURG,GERMANY
EICHMANN, K
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SAIZAWA, MK
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MAX PLANCK INST IMMUNBIOL,W-7800 FREIBURG,GERMANYMAX PLANCK INST IMMUNBIOL,W-7800 FREIBURG,GERMANY
SAIZAWA, MK
[1
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[1] MAX PLANCK INST IMMUNBIOL,W-7800 FREIBURG,GERMANY
The association of components of the CD3 complex with the accessory molecules CD4 and CD8 was studied by immunoprecipitation experiments followed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) analysis. Enhanced surface iodination was achieved by a water-soluble derivative of the Bolton-Hunter reagent. Using freshly isolated nonactivated splenic T cells, we find that antibodies to CD4 and to CD8 strongly co-precipitate a 28-30-kDa band identical in mobility to the delta chain of the CD3 complex. Components corresponding in mobility to the epsilon and gamma chains of the CD3 complex are also co-precipitated but to a much lesser extent. The identity of the co-precipitated 28-30-kDa material with the CD3 delta chain was ascertained by two-dimensional nonreducing/reducing SDS-PAGE, by two-dimensional non-equilibrium pH gradient electrophoresis/SDS-PAGE and by one-dimensional peptide mapping with three different proteases. The co-precipitated 28-30-kDa material was identical to the CD3 delta chain by all these criteria. Quantitative analyses by densitometric gel tracing revealed that the amounts of CD3 delta co-precipitated with anti-CD4 and anti-CD8 add up to those in anti-V(beta) precipitates and to an average of 90% of those in anti-CD3epsilon precipitates.We conclude that the majority of CD3 delta chains are associated with the accessory/co-receptor molecules CD4 or CD8 on resting T cells, and that this association is independent of antigen-specific recognition by the T cell receptor.
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STANFORD UNIV, MED CTR, SCH MED, DEPT MED MICROBIOL, STANFORD, CA 94305 USASTANFORD UNIV, MED CTR, SCH MED, DEPT MED MICROBIOL, STANFORD, CA 94305 USA
GALLAGHER, PF
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FAZEKAS DE ST GROTH, B
MILLER, JFAP
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STANFORD UNIV, MED CTR, SCH MED, DEPT MED MICROBIOL, STANFORD, CA 94305 USASTANFORD UNIV, MED CTR, SCH MED, DEPT MED MICROBIOL, STANFORD, CA 94305 USA
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STANFORD UNIV, MED CTR, SCH MED, DEPT MED MICROBIOL, STANFORD, CA 94305 USASTANFORD UNIV, MED CTR, SCH MED, DEPT MED MICROBIOL, STANFORD, CA 94305 USA
GALLAGHER, PF
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FAZEKAS DE ST GROTH, B
MILLER, JFAP
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STANFORD UNIV, MED CTR, SCH MED, DEPT MED MICROBIOL, STANFORD, CA 94305 USASTANFORD UNIV, MED CTR, SCH MED, DEPT MED MICROBIOL, STANFORD, CA 94305 USA