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有丝分裂原对静息淋巴细胞的激活会暴露隐藏的胰岛素受体。

Mitogen activation of resting lymphocytes exposes cryptic insulin receptors.

作者信息

Goodman D W, Isakson P C

机构信息

Department of Pharmacology, University of Virginia Health Sciences Center, Charlottesville 22908.

出版信息

J Biol Chem. 1993 Feb 25;268(6):4207-15.

PMID:8440705
Abstract

Mitogen activation of resting lymphocytes induces expression of high affinity insulin receptors on the plasma membrane. The mechanism underlying this effect on insulin receptor expression was examined by comparing levels of insulin receptor mRNA and protein in resting and mitogen-activated rodent lymphocytes. Analysis of RNA levels indicated that resting and concanavalin A-activated lymphocytes contained equivalent amounts of insulin receptor mRNA with predominant transcripts of 7.9 and 9.5 kilobases. Although little or no insulin binding was detectable on intact resting lymphocytes, detergent solubilization of these cells resulted in the appearance of readily detectable insulin binding activity that could be immunoprecipitated with anti-insulin receptor antibodies. Detergent-solubilized resting and mitogen-activated lymphocytes expressed equivalent amounts of insulin receptors that bound insulin with similar affinity (KD = 90 pM) and migrated on reduced SDS-polyacrylamide gels with apparent masses of approximately 130 and approximately 95 kDa. Insulin receptors from resting lymphocytes appeared to be associated with the plasma membrane since 125I labeling of intact lymphocytes radiolabeled the insulin receptor, insulin binding activity was detected in membrane fractions of hypotonically lysed cells, and trypsin treatment of intact cells destroyed > 90% of the insulin binding activity in detergent extracts. These results suggest that resting lymphocytes express insulin receptor mRNA and protein and that mitogen activation exposes cryptic insulin receptors present in the plasma membrane of resting lymphocytes.

摘要

静息淋巴细胞的丝裂原激活可诱导质膜上高亲和力胰岛素受体的表达。通过比较静息和丝裂原激活的啮齿动物淋巴细胞中胰岛素受体mRNA和蛋白质的水平,研究了这种对胰岛素受体表达影响的潜在机制。RNA水平分析表明,静息和伴刀豆球蛋白A激活的淋巴细胞含有等量的胰岛素受体mRNA,主要转录本为7.9和9.5千碱基。虽然在完整的静息淋巴细胞上几乎检测不到胰岛素结合,但这些细胞的去污剂溶解导致出现易于检测的胰岛素结合活性,该活性可用抗胰岛素受体抗体进行免疫沉淀。去污剂溶解的静息和丝裂原激活的淋巴细胞表达等量的胰岛素受体,这些受体以相似的亲和力(KD = 90 pM)结合胰岛素,并在还原的SDS-聚丙烯酰胺凝胶上迁移,表观分子量约为130 kDa和约95 kDa。静息淋巴细胞的胰岛素受体似乎与质膜相关,因为完整淋巴细胞的125I标记可使胰岛素受体放射性标记,在低渗裂解细胞的膜部分检测到胰岛素结合活性,并且对完整细胞进行胰蛋白酶处理可破坏去污剂提取物中> 90%的胰岛素结合活性。这些结果表明,静息淋巴细胞表达胰岛素受体mRNA和蛋白质,并且丝裂原激活暴露了静息淋巴细胞质膜中存在的隐蔽胰岛素受体。

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