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人巨噬细胞集落刺激因子(M-CSF):可变RNA剪接产生三种不同的蛋白质,它们在细胞表面表达并分泌。

Human macrophage colony stimulating factor (M-CSF): alternate RNA splicing generates three different proteins that are expressed on the cell surface and secreted.

作者信息

Cosman D, Wignall J, Anderson D, Tushinski J, Gallis B, Urdal D, Cerretti D P

机构信息

Department of Molecular Biology, Immunex Corporation, Seattle, Washington 98101.

出版信息

Behring Inst Mitt. 1988 Aug(83):15-26.

PMID:3071332
Abstract

Human macrophage colony stimulating factor (M-CSF) cDNA clones were isolated from a pancreatic carcinoma cell line. Three different classes of M-CSF precursor protein (256, 554 and 438 amino acids in length) were predicted to be encoded by these cDNAs. Two of these, that we designate M-CSF alpha and M-CSF beta have already been described. The third, M-CSF gamma represents a novel class of M-CSF cDNA. All three precursors share a 32 amino acid signal sequence and the first 149 amino acids of the mature protein. At this position, M-CSF beta and gamma have insertions of 298 and 182 amino acids relative to M-CSF alpha. The first 182 amino acids of these insertions are shared between M-CSF beta and gamma. All three precursors share the C-terminal 75 amino acids that encode the transmembrane and cytoplasmic domains. Expression of all three cDNAs in COS-7 monkey kidney cells gave rise to soluble M-CSF activity, associated with proteins of subunit molecular weight 44 Kda (beta and gamma) or 28 Kda (alpha). In addition, M-CSF proteins could be detected on the surface of the transfected cells by indirect immunofluorescence. When the transmembrane and cytoplasmic domains of M-CSF alpha were removed by introducing a stop codon after amino acid 190, no membrane-bound M-CSF could be detected, but the truncated protein was secreted efficiently and was biologically active. This suggests that all three forms of M-CSF can exist as cell surface proteins, anchored by their hydrophobic transmembrane domains, and can be processed to soluble forms by proteolytic digestion. Although all soluble forms of M-CSF were biologically active in murine bone marrow colony and proliferation assays, they showed greatly reduced or no activity in similar assays using human bone marrow.

摘要

从胰腺癌细胞系中分离出了人巨噬细胞集落刺激因子(M-CSF)的cDNA克隆。预计这些cDNA可编码三种不同类型的M-CSF前体蛋白(长度分别为256、554和438个氨基酸)。其中两种,即我们命名的M-CSFα和M-CSFβ,此前已有描述。第三种,M-CSFγ代表一类新型的M-CSF cDNA。所有这三种前体都有一个32个氨基酸的信号序列以及成熟蛋白的前149个氨基酸。在这个位置,相对于M-CSFα,M-CSFβ和γ分别有298和182个氨基酸的插入。这些插入的前182个氨基酸在M-CSFβ和γ之间是相同的。所有这三种前体都共享编码跨膜和胞质结构域的C末端75个氨基酸。在COS-7猴肾细胞中表达所有这三种cDNA,均产生了可溶性M-CSF活性,这与亚基分子量为44 kDa(β和γ)或28 kDa(α)的蛋白质相关。此外,通过间接免疫荧光可在转染细胞表面检测到M-CSF蛋白。当通过在第190位氨基酸后引入终止密码子去除M-CSFα的跨膜和胞质结构域时,未检测到膜结合的M-CSF,但截短的蛋白被有效分泌且具有生物活性。这表明所有三种形式的M-CSF都可以作为细胞表面蛋白存在,通过其疏水的跨膜结构域锚定,并可通过蛋白水解切割加工成可溶性形式。尽管所有可溶性形式的M-CSF在小鼠骨髓集落和增殖试验中具有生物活性,但在使用人骨髓的类似试验中,它们的活性大大降低或无活性。

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Behring Inst Mitt. 1988 Aug(83):15-26.
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