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对成红细胞转化有缺陷的禽成红细胞增多症病毒突变体:p75的erb部分缺失表明该蛋白在白血病发生中的作用。

Mutant of avian erythroblastosis virus defective for erythroblast transformation: deletion in the erb portion of p75 suggests function of the protein in leukemogenesis.

作者信息

Beug H, Kitchener G, Doederlein G, Graf T, Hayman M J

出版信息

Proc Natl Acad Sci U S A. 1980 Nov;77(11):6683-6. doi: 10.1073/pnas.77.11.6683.

Abstract

Previous studies have shown that td359 AEV, a mutant of avian erythroblastosis virus (AEV), is unable to transform erythroblasts in vitro or in vivo but is capable of transforming fibroblasts in vitro and of causing sarcomas in chicks. In this paper we show that the mutant synthesizes a gag-gene related protein (delta p75) which is about 1000 daltons smaller than the protein, p75, induced by wild-type AEV. The mutant protein lacks 3 of the approximately 53 lysine-arginine tryptic peptides resolved in p75 and also contains an additional peptide. By cleavage of delta p75 with p15 protease and analysis of the fragments for size and peptide composition, the deletion in delta p75 could be located in the non-gag region of the molecule. In contrast, with p40 AEV, a second AEV-specific protein synthesized in in vitro translation experiments, there is no change in size of translation products obtained from td359 AEV RNA. Our data provide direct evidence that p75 is required for erythroblast transformation.

摘要

先前的研究表明,禽成红细胞增多症病毒(AEV)的突变体td359 AEV在体外或体内均无法转化成红细胞,但能够在体外转化成纤维细胞并在雏鸡中引发肉瘤。在本文中,我们表明该突变体合成了一种与gag基因相关的蛋白质(δp75),其比野生型AEV诱导产生的蛋白质p75小约1000道尔顿。突变蛋白缺少p75中分辨出的约53个赖氨酸 - 精氨酸胰蛋白酶肽中的3个,并且还包含一个额外的肽段。通过用p15蛋白酶切割δp75并分析片段的大小和肽组成,δp75中的缺失可定位在分子的非gag区域。相比之下,对于p40 AEV(在体外翻译实验中合成的第二种AEV特异性蛋白质),从td359 AEV RNA获得的翻译产物大小没有变化。我们的数据提供了直接证据,证明p75是成红细胞转化所必需的。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/db87/350352/46cdfc9bd216/pnas00498-0437-a.jpg

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