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禽逆转录病毒逆转录酶和核酸内切酶结构域的结构表征。

Structural characterization of the avian retrovirus reverse transcriptase and endonuclease domains.

作者信息

Grandgenett D, Quinn T, Hippenmeyer P J, Oroszlan S

出版信息

J Biol Chem. 1985 Jul 15;260(14):8243-9.

PMID:2989284
Abstract

The enzymatic domains of the avian retrovirus polymerase (pol) gene have been mapped by the use of peptide antibodies and COOH-terminal amino acid analysis. The processed pol beta polypeptide is cleaved in vivo to yield alpha and pp32. Rabbit antibodies were directed against synthetic peptides whose sequence was deduced from the known pol sequence of Rous sarcoma virus, Prague C (Schwartz, D.E., Tizard, R., and Gilbert, W. (1983) Cell 32, 853-869). The RNase H active site of pol was located in the NH2-terminal region of the alpha DNA polymerase subunit. The COOH terminus of the alpha subunit was found to be immediately adjacent to the NH2 terminus of the pp32 pol protein. COOH-terminal amino acid analysis of pp32 revealed that this protein is also processed. From the deduced amino acid sequence of pol, it appears likely that pol encodes an additional 4100-dalton polypeptide located at its extreme COOH terminus. The enzymatic domains on beta appear to map in the following order: RNase H-DNA polymerase-DNA endonuclease. Hydrophilicity analysis and secondary structure predictions of wild type Rous sarcoma virus pol products and mutated pp32 possessing single amino acid changes permit further structural evaluation of the multifunctional pol protein.

摘要

利用肽抗体和羧基末端氨基酸分析对禽逆转录病毒聚合酶(pol)基因的酶结构域进行了定位。加工后的polβ多肽在体内被切割,产生α和pp32。兔抗体针对的是合成肽,其序列是根据劳氏肉瘤病毒布拉格C株已知的pol序列推导出来的(施瓦茨,D.E.,蒂扎德,R.,和吉尔伯特,W.(1983年)《细胞》32卷,853 - 869页)。pol的核糖核酸酶H活性位点位于αDNA聚合酶亚基的氨基末端区域。发现α亚基的羧基末端紧邻pp32 pol蛋白的氨基末端。对pp32的羧基末端氨基酸分析表明该蛋白也经过了加工。从pol推导的氨基酸序列来看,pol似乎在其极端羧基末端编码一种额外的4100道尔顿的多肽。β上的酶结构域似乎按以下顺序定位:核糖核酸酶H - DNA聚合酶 - DNA内切酶。对野生型劳氏肉瘤病毒pol产物和具有单个氨基酸变化的突变型pp32进行亲水性分析和二级结构预测,有助于对多功能pol蛋白进行进一步的结构评估。

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