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通过使用5-溴脱氧尿苷进行光交联鉴定的端粒蛋白-DNA点接触。

Telomeric protein-DNA point contacts identified by photo-cross-linking using 5-bromodeoxyuridine.

作者信息

Hicke B J, Willis M C, Koch T H, Cech T R

机构信息

Department of Molecular, Cellular, and Developmental Biology, Howard Hughes Medical Institute, University of Colorado, Boulder 80309-0215.

出版信息

Biochemistry. 1994 Mar 22;33(11):3364-73. doi: 10.1021/bi00177a030.

Abstract

The Oxytricha telomere protein specifically recognizes single-stranded telomeric DNA, forming an extremely salt resistant and kinetically stable nucleoprotein complex. The absence of information on how this heterodimeric protein binds to DNA prompted this photo-cross-linking study. Multiple protein-DNA photo-cross-links are formed upon UV irradiation of Oxytricha telomeres reconstituted with a synthetic oligonucleotide terminating in 5'-T16T15T14T13G12G11G10G9T8T7T6T5G4G3G2G1-3'. Site-specific substitution of certain nucleotides with 5-bromodeoxyuridine (BrdU) greatly increased the photo-cross-linking yield, each substitution favoring a specific protein-DNA cross-link. For example, substitution of BrdU for T7 resulted in 25% cross-linking of the bound DNA, a 10-fold increase over the unsubstituted DNA. Both subunits of the telomere protein cross-link to, and are therefore near, the DNA. Three point contacts within this nucleoprotein complex, involving the alpha subunit, were established using BrdU substitution: Tyr239, Tyr142, and His292 cross-link to G3, T15, and T7, respectively. One photo-cross-link, Tyr239-G3, occurs amid a short acidic stretch of the alpha subunit, counter to expectations for amino acids that approach the polyanionic DNA. The two remaining cross-links are to amino acids in hydrophobic regions of the primary polypeptide sequence, consistent with the hypothesis that hydrophobic interactions account for the salt resistance (> 2 M NaCl) of this protein-DNA complex. These two photo-cross-links suggest that the telomere protein may bind telomeric single-stranded DNA by intercalation of aromatic residues into a nucleotide lattice.

摘要

嗜热四膜虫端粒蛋白能特异性识别单链端粒DNA,形成一种极具耐盐性且动力学稳定的核蛋白复合物。由于缺乏关于这种异二聚体蛋白如何与DNA结合的信息,促使我们开展了这项光交联研究。用5'-T16T15T14T13G12G11G10G9T8T7T6T5G4G3G2G1-3'末端的合成寡核苷酸重建嗜热四膜虫端粒,经紫外线照射后会形成多个蛋白质-DNA光交联。用5-溴脱氧尿苷(BrdU)对某些核苷酸进行位点特异性取代,极大地提高了光交联产率,每次取代都有利于形成特定的蛋白质-DNA交联。例如,用BrdU取代T7会导致25%的结合DNA发生交联,比未取代的DNA增加了10倍。端粒蛋白的两个亚基都与DNA发生交联,因此靠近DNA。利用BrdU取代确定了该核蛋白复合物中涉及α亚基的三个点接触:Tyr239、Tyr142和His292分别与G3、T15和T7交联。一个光交联Tyr239-G3发生在α亚基的一段短酸性区域内,这与接近多阴离子DNA的氨基酸的预期情况相反。其余两个交联发生在一级多肽序列疏水区域的氨基酸上,这与疏水相互作用导致该蛋白质-DNA复合物具有耐盐性(>2M NaCl)的假设一致。这两个光交联表明,端粒蛋白可能通过将芳香族残基插入核苷酸晶格来结合端粒单链DNA。

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