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Comparative tryptic peptide mapping studies suggest a role in cell transformation for the gag-related protein of avian erythroblastosis virus and avian myelocytomatosis virus strains CMII and MC29.

机译:比较性的胰蛋白酶肽图研究表明,禽红细胞母细胞增生病毒和禽骨髓瘤细胞增生病毒株CMII和MC29的gag相关蛋白在细胞转化中起作用。

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摘要

The gag-related proteins found in cells transformed by avian erythroblastosis virus (AEV) and the avian myelocytomatosis viruses MC29 and CMII have been compared by tryptic peptide fingerprinting. A comparison of the methionine-containing tryptic peptides of the AEV 75-kilodalton protein, the CMII 90-kilodalton protein, and the MC29 110-kilodalton protein with the gag gene product Pr76 of their naturally occurring helper leukemia viruses enabled us to distinguish those peptides related to the gag gene from the non-gag-related peptides. The 12 non-gag peptides found in the AEV 75-kilodalton protein were unique to this protein and not found in the MC29 110-kilodalton or CMII 90-kilodalton proteins. In contrast, the MC29 110-kilodalton protein shared two methionine-containing non-gag tryptic peptides with the CMII 90-kilodalton protein. When these experiments were repeated with [14C]lysine and [14C]arginine as the labeled amino acids, the MC29 110-kilodalton protein and the CMII 90-kilodalton protein were found to share 30 out of approximately 40 non-gag-related peptides. These results demonstrate that viruses with a similar transformation spectrum synthesize related proteins and suggest that the gag-related proteins represent the transforming proteins of the replication-defective avian leukemia viruses.
机译:已通过胰蛋白酶肽指纹图谱比较了在禽红细胞母细胞增生病毒(AEV)和禽骨髓细胞瘤病毒MC29和CMII转化的细胞中发现的与gag相关的蛋白质。将AEV 75-千洛顿蛋白,CMII 90-千洛顿蛋白和MC29 110-千洛顿蛋白的含蛋氨酸胰蛋白酶肽与它们的天然辅助性白血病病毒的gag基因产物Pr76进行比较,使我们能够区分这些肽与非gag相关肽的gag基因有关。在AEV 75千达尔顿蛋白中发现的12个非gag肽对该蛋白是唯一的,而在MC29 110千达尔顿或CMII 90千达尔顿蛋白中没有。相反,MC29 110-千达尔顿蛋白与CMII 90-千达尔顿蛋白共享两个含蛋氨酸的非gag胰蛋白酶肽。当用[14C]赖氨酸和[14C]精氨酸作为标记的氨基酸重复这些实验时,发现MC29 110-千达尔顿蛋白和CMII 90-千达尔顿蛋白共享约40个非gag相关肽中的30个。这些结果表明,具有相似转化谱的病毒可以合成相关蛋白,并表明gag相关蛋白代表复制缺陷型禽白血病病毒的转化蛋白。

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    Kitchener, G; Hayman, M J;

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