Green M, Symington J, Brackmann K H, Cartas M A, Thornton H, Young L
J Virol. 1981 Nov;40(2):541-50. doi: 10.1128/JVI.40.2.541-550.1981.
Highly purified adenovirus type 2 terminal protein (TP) with an apparent M(r) of 55,000 (55K) was prepared in quantities of 10 to 30 mug from guanidine hydrochloride- or sodium dodecyl sulfate-disrupted virions (60 to 120 mg). Guinea pigs were immunized with 14 to 20 injections of TP in amounts of 1 to 2 mug. Antiserum to TP was used to study the intracellular polypeptides related to adenovirus type 2 TP. By immunoprecipitation with anti-TP serum, we identified 80K and 76K polypeptides in the nucleoplasmic and cytoplasmic S100 fractions of [(35)S]methionine-labeled cells early and late after infection with Ad2. By immunoautoradiographic analysis which eliminates coprecipitation of unrelated proteins, we identified an 80K polypeptide (probably an 80K-76K doublet) in unlabeled, late infected cells, using anti-TP serum and (125)I-labeled staphylococcal protein A. About two- to threefold-higher levels of the 80K and 76K polypeptides were present in the nucleoplasm than in the S100 fraction, and two- to threefold-higher levels were found in late infected cells than in early infected cells (cycloheximide enhanced, arabinofuranosylcytosine treated). We did not detect the 80K or 76K polypeptide in uninfected cells, indicating that these polypeptides are virus coded. Tryptic peptide map analysis showed that the 80K and 76K polypeptides are very closely related and that they share peptides with the DNA-bound 55K TP. Our data provide the first direct demonstration of intracellular 80K and 76K forms of TP. The intracellular 80K and 76K polypeptides are closely related or identical to the 80K polypeptide that Challberg and co-workers (Proc. Natl. Acad. Sci. U.S.A. 77:5105-5109, 1980) detected at the termini of adenovirus DNA synthesized in vitro and to the 87K polypeptide that Stillman and co-workers (Cell 23:497-508, 1981) translated in vitro. We did not detect the 55K TP in early or late infected cells, consistent with the proposal by Challberg and co-workers that the 80K polypeptide is a precursor to the virion-bound TP and that the conversion of the 80K polypeptide to the 55K TP occurs during virus maturation. The 80K and 76K polypeptides have many more methionine-containing tryptic peptides than does the 55K TP, and most of the tryptic peptides unique to the 80K and 76K polypeptides are very hydrophobic. Thus, the conversion of the 80K and 76K polypeptides to the 55K TP may involve the removal of a specific hydrophobic protein region.
从盐酸胍或十二烷基硫酸钠裂解的病毒粒子(60至120毫克)中制备出了表观分子量为55,000(55K)的高纯度2型腺病毒末端蛋白(TP),产量为10至30微克。用1至2微克的TP对豚鼠进行14至20次注射免疫。用TP抗血清研究与2型腺病毒TP相关的细胞内多肽。通过用抗TP血清进行免疫沉淀,我们在感染Ad2的早期和晚期,在[³⁵S]甲硫氨酸标记细胞的核质和细胞质S100组分中鉴定出了80K和76K多肽。通过免疫放射自显影分析(消除无关蛋白的共沉淀),我们使用抗TP血清和¹²⁵I标记的葡萄球菌蛋白A,在未标记的晚期感染细胞中鉴定出了一种80K多肽(可能是80K - 76K双峰)。核质中80K和76K多肽的水平比S100组分中的高约两到三倍,晚期感染细胞中的水平比早期感染细胞中的高两到三倍(环己酰亚胺增强,经阿糖胞苷处理)。我们在未感染细胞中未检测到80K或76K多肽,这表明这些多肽是病毒编码的。胰蛋白酶肽图谱分析表明,80K和76K多肽密切相关,并且它们与结合DNA的55K TP共享肽段。我们的数据首次直接证明了细胞内存在80K和76K形式的TP。细胞内的80K和76K多肽与Challberg及其同事(《美国国家科学院院刊》77:5105 - 5109,1980)在体外合成的腺病毒DNA末端检测到的80K多肽以及Stillman及其同事(《细胞》23:497 - 508,1981)在体外翻译的87K多肽密切相关或相同。我们在早期或晚期感染细胞中均未检测到55K TP,这与Challberg及其同事的提议一致,即80K多肽是病毒粒子结合TP的前体,并且80K多肽向55K TP的转化发生在病毒成熟过程中。80K和76K多肽含甲硫氨酸的胰蛋白酶肽段比55K TP多得多,并且80K和76K多肽特有的大多数胰蛋白酶肽段非常疏水。因此,80K和76K多肽向55K TP的转化可能涉及去除特定的疏水蛋白区域。
