Receptors for T cell-replacing factor/interleukin 5. Specificity, quantitation, and its implication.
10.1084/jem.168.3.863
Crossref journal-article
Rockefeller University Press
The Journal of experimental medicine (291)
Abstract

T cell-replacing factor (TRF)/IL-5 is a glycosylated polypeptide that acts as a key factor for B cell growth and differentiation. Since IL-5 action is probably mediated by specific cell surface receptor(s), we have characterized the binding of IL-5 to cells using biosynthetically [35S]methionine-labeled IL-5 and 125I-IL-5 that had been prepared using Bolton-Hunter reagent. The radiolabeled IL-5 binds specifically to BCL1-B20 (in vitro line) (a murine chronic B cell leukemic cell line previously shown to differentiate into IgM-secreting cells in response to IL-5) within 10 min at 37 degrees C. There are two classes of binding sites with high affinity (Kd = 66 pM) and low affinity (Kd = 12 nM) for IL-5 and an average number of binding sites for high affinity and for low affinity were 400 and 7,500 per cell, respectively. The specificity of binding of radiolabeled IL-5 has been confirmed by demonstrating that only unlabeled IL-5 and anti-IL-5 mAb but not by IL-1, IL-2, IL-3, IFN-gamma, and GM-CSF inhibit radiolabeled IL-5 binding to BCL1-B20 cells. Treatment of surface-bound radiolabeled IL-5 with bivalent crosslinkers identified a membrane polypeptide of Mr 46,500 to which IL-5 is crosslinked. A variety of cell types have been surveyed for the capacity to bind specifically radiolabeled IL-5 with high affinity. BCL1 cells MOPC104E (murine myeloma cell line) expressed IL-5-R, whereas BAL. 17 and L10 A (B cell lymphoma) did not. T cell line, mastocytoma cell line, or macrophage tumor cell line did not display detectable levels of IL-5-R. were hardly detectable on normal resting B cells but were expressed on LPS-activated B cells, fitting the function of IL-5 that acts on activated B cells for their differentiation into Ig-secreting cells. Intriguingly, early B cell lines (J-87 and T-88) that grow in the presence of IL-5 expressed significant but low numbers of high-affinity binding sites for IL-5. The biological effects of IL-5 were mediated by high-affinity binding sites. The identification and characterization of IL-5-R should provide new insight into the apparent diverse biological activities of IL-5.

Bibliography

Mita, S., Harada, N., Naomi, S., Hitoshi, Y., Sakamoto, K., Akagi, M., Tominaga, A., & Takatsu, K. (1988). Receptors for T cell-replacing factor/interleukin 5. Specificity, quantitation, and its implication. The Journal of Experimental Medicine, 168(3), 863–878.

Authors 8
  1. S Mita (first)
  2. N Harada (additional)
  3. S Naomi (additional)
  4. Y Hitoshi (additional)
  5. K Sakamoto (additional)
  6. M Akagi (additional)
  7. A Tominaga (additional)
  8. K Takatsu (additional)
References 0 Referenced 59

None

Dates
Type When
Created 21 years, 2 months ago (June 24, 2004, 3:56 a.m.)
Deposited 2 years, 1 month ago (July 24, 2023, 9:22 p.m.)
Indexed 5 months ago (March 31, 2025, 9:23 a.m.)
Issued 37 years ago (Sept. 1, 1988)
Published 37 years ago (Sept. 1, 1988)
Published Online 37 years ago (Sept. 1, 1988)
Published Print 37 years ago (Sept. 1, 1988)
Funders 0

None

@article{Mita_1988, title={Receptors for T cell-replacing factor/interleukin 5. Specificity, quantitation, and its implication.}, volume={168}, ISSN={1540-9538}, url={http://dx.doi.org/10.1084/jem.168.3.863}, DOI={10.1084/jem.168.3.863}, number={3}, journal={The Journal of experimental medicine}, publisher={Rockefeller University Press}, author={Mita, S and Harada, N and Naomi, S and Hitoshi, Y and Sakamoto, K and Akagi, M and Tominaga, A and Takatsu, K}, year={1988}, month=sep, pages={863–878} }