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Identification of a cDNA for a human high-molecular-weight B-cell growth factor

  • Julian L. Ambrus
  • , James Pippin
  • , Amy Joseph
  • , Chenguang Xu
  • , David Blumenthal
  • , Archi Tamayo
  • , Kent Claypool
  • , David Mccourt
  • , Anon Srikiatchatochorn
  • , Richard J. Ford
  • Washington University St. Louis
  • University of Texas MD Anderson Cancer Center

Research output: Contribution to journalArticlepeer-review

45 Scopus citations

Abstract

Proliferation is necessary for many of the phenotypic changes that occur during B-cell maturation. Further differentiation of mature B cells into plasma cells or memory B cells requires additional rounds of proliferation. In this manuscript, we describe a cDNA for a human B-cell growth factor we call high-molecular-weight B-cell growth factor (HMW-BCGF). Purified HMW-BCGF has been shown to induce B-cell proliferation, inhibit immunoglobulin secretion, and selectively expand certain B-cell subpopulations. Studies using antibodies to HMW-BCGF and its receptor have suggested that HMW-BCGF, while produced by T cells and some malignant B cells, acts predominantly on normal and malignant B cells. The HMW-BCGF cDNA was identified by expression cloning using a monoclonal antibody and polyclonal antisera to HMW-BCGF. Protein produced from the cDNA induced B-cell proliferation, inhibited immunoglobulin secretion, and was recognized in immunoblots by anti-HMW-BCGF antibodies. The amino acid sequence of HMW-BCGF deduced from the cDNA predicts a secreted protein of 53 kDa with three potential N-linked glycosylation sites. The identification of this cDNA will allow further studies examining physiologic roles of this cytokine. We propose to call it interleukin 14.

Original languageEnglish
Pages (from-to)6330-6334
Number of pages5
JournalProceedings of the National Academy of Sciences of the United States of America
Volume90
Issue number13
StatePublished - Jul 1 1993

Keywords

  • Cytokine
  • Growth factor
  • Interleukin
  • Leukemia
  • Lymphoma

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