Farrar Y J, Evans R K, Beach C M, Coleman M S
Department of Biochemistry, University of Kentucky, Lexington 40536-0084.
Biochemistry. 1991 Mar 26;30(12):3075-82. doi: 10.1021/bi00226a014.
Terminal deoxynucleotidyl transferase (terminal transferase) was specifically modified in the DNA binding site by a photoactive DNA substrate (hetero-40-mer duplex containing eight 5-azido-dUMP residues at one 3' end). Under optimal photolabeling conditions, 27-40% of the DNA was covalently cross-linked to terminal transferase. The specificity of the DNA and protein interaction was demonstrated by protection of photolabeling at the DNA binding domain with natural DNA substrates. In order to recover high yields of modified peptides from limited amounts of starting material, protein modified with 32P-labeled photoactive DNA and digested with trypsin was extracted 4 times with phenol followed by gel filtration chromatography. All peptides not cross-linked to DNA were extracted into the phenol phase while the photolyzed DNA and the covalently cross-linked peptides remained in the aqueous phase. The 32P-containing peptide-DNA fraction was subjected to amino acid sequence analysis. Two sequences, Asp221-Lys231 (peptide B8) and Cys234-Lys249 (peptide B10), present in similar yield, were identified. Structure predictions placed the two peptides in an alpha-helical array of 39 A which would accommodate a DNA helix span of 11 nucleotides. These peptides share sequence similarity with a region in DNA polymerase beta that has been implicated in the binding of DNA template.
末端脱氧核苷酸转移酶(末端转移酶)通过一种光活性DNA底物(一种在3'末端含有八个5-叠氮基-dUMP残基的异源40聚体双链体)在DNA结合位点进行特异性修饰。在最佳光标记条件下,27% - 40%的DNA与末端转移酶发生共价交联。天然DNA底物对DNA结合结构域光标记的保护作用证明了DNA与蛋白质相互作用的特异性。为了从有限量的起始材料中获得高产率的修饰肽,用32P标记的光活性DNA修饰并经胰蛋白酶消化的蛋白质先用苯酚萃取4次,然后进行凝胶过滤色谱。所有未与DNA交联的肽都被萃取到苯酚相中,而光解的DNA和共价交联的肽则保留在水相中。对含32P的肽 - DNA组分进行氨基酸序列分析。鉴定出两条产量相似的序列,即Asp221 - Lys231(肽B8)和Cys234 - Lys249(肽B10)。结构预测将这两条肽置于一个39 Å的α螺旋阵列中,该阵列可容纳一个11个核苷酸的DNA螺旋跨度。这些肽与DNA聚合酶β中一个与DNA模板结合有关的区域具有序列相似性。
