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骨髓基质细胞和白细胞介素-7诱导BP-1/6C3抗原的协同表达和前B细胞生长。

Bone marrow stromal cells and interleukin-7 induce coordinate expression of the BP-1/6C3 antigen and pre-B cell growth.

作者信息

Welch P A, Burrows P D, Namen A, Gillis S, Cooper M D

机构信息

Division of Developmental and Clinical Immunology, University of Alabama, Birmingham 35294.

出版信息

Int Immunol. 1990;2(8):697-705. doi: 10.1093/intimm/2.8.697.

DOI:10.1093/intimm/2.8.697
PMID:2083232
Abstract

The BP-1/6C3 molecule expressed by early B lineage cells and some stromal cells is a type II integral membrane glycoprotein that belongs to the zinc-dependent family of metallopeptidases. In order to explore the potential role of this cell surface molecule in precursor B cell proliferation, we established a stromal cell line (BHM) from long-term bone marrow cultures of the Whitlock - Witte type and developed a rapid bioassay for the detection of responsive target cells. When non-adherent bone marrow cells were cultured with BHM stroma, we observed an up-regulation of BP-1 expression by the B cell precursors that coincided with the induction of proliferation. The precursor B-cell targets included bone marrow cells that lacked detectable BP-1/6C3, B220, and Ia antigens. They could be identified in fetal liver and in the bone marrow, but not the thymus, spleen, or lymph nodes, of normal BALB/c mice, and were also present in the bone marrow of mice with the nu/nu, CBA/N, and SCID defects. Because the inductive effects on precursor B cells could be reproduced with BHM supernatant, soluble growth factors were evaluated in the assay. Interleukin 7 (IL-7) appeared to be unique in its ability to induce BP-1/6C3 expression and concomitant cell growth. Northern blot analysis revealed that the BHM stromal cells, which themselves express the BP-1 antigen, constitutively expressed high levels of variable length transcripts for IL-7. The data suggest that the IL-7 product of stromal cells selectively induces BP-1/6C3 expression on B cell precursors and may implicate this cell surface glycoprotein in the control of IL-7 induced proliferation of early B lineage cells.

摘要

早期B淋巴细胞系细胞和一些基质细胞表达的BP-1/6C3分子是一种II型整合膜糖蛋白,属于金属肽酶的锌依赖家族。为了探究这种细胞表面分子在前体B细胞增殖中的潜在作用,我们从Whitlock-Witte型长期骨髓培养物中建立了一种基质细胞系(BHM),并开发了一种用于检测反应性靶细胞的快速生物测定法。当非贴壁骨髓细胞与BHM基质共同培养时,我们观察到B细胞前体的BP-1表达上调,这与增殖的诱导同时发生。前体B细胞靶标包括缺乏可检测到的BP-1/6C3、B220和Ia抗原的骨髓细胞。它们可在正常BALB/c小鼠的胎肝和骨髓中被识别,但在胸腺、脾脏或淋巴结中未被识别,并且也存在于具有nu/nu、CBA/N和SCID缺陷的小鼠的骨髓中。因为对前体B细胞的诱导作用可用BHM上清液重现,所以在该测定法中对可溶性生长因子进行了评估。白细胞介素7(IL-7)在诱导BP-1/6C3表达和伴随的细胞生长方面似乎具有独特能力。Northern印迹分析显示,本身表达BP-1抗原的BHM基质细胞组成性地高水平表达可变长度的IL-7转录本。数据表明,基质细胞的IL-7产物选择性地诱导B细胞前体上的BP-1/6C3表达,并且可能表明这种细胞表面糖蛋白参与了IL-7诱导的早期B淋巴细胞系细胞增殖的控制。

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