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紫外线诱导的信使核糖核酸与蛋白质的交联

Ultraviolet light-induced crosslinking of mRNA to proteins.

作者信息

Greenberg J R

出版信息

Nucleic Acids Res. 1979 Feb;6(2):715-32. doi: 10.1093/nar/6.2.715.

Abstract

Irradiation of intact or EDTA-dissociated L-cell polyribosomes with 254 nm UV light at doses of 1-2 x 10(5) ergs/mm2 extensively crosslinks mRNA to proteins. The crosslinked mRNA-protein complexes can be isolated on the basis of buoyant density in urea-containing CS2SO4 gradients that dissociate non-covalent complexes. Crosslinking of mRNA can also be assayed by phenolchloroform extraction. mRNA recovered from the crosslinked complexes by digestion with proteinase K has the same electrophoretic mobility in polyacrylamide gels as unirradiated mRNA. Therefore, irradiation does not either crosslink RNA molecules to RNA molecules or break phosphodiester bonds. With these methods it has been found that more than 70% of high molecular weight polydisperse mRNA, but only 25-40% of histone mRNA, can be crosslinked to protein. On the basis of buoyant density the histone mRNA-protein complex had a protein content of 26%, whereas the mean protein content of most non-histone mRNA-protein complexes was 65%. It is concluded that most mRNA in polyribosomes is in close contact with proteins, and that histone mRNA can be crosslinked to many fewer proteins that most other mRNAs.

摘要

用剂量为1 - 2×10⁵尔格/平方毫米的254纳米紫外线照射完整的或经乙二胺四乙酸(EDTA)解离的L细胞多核糖体,会使信使核糖核酸(mRNA)与蛋白质广泛交联。交联的mRNA - 蛋白质复合物可根据其在含尿素的硫酸铯(Cs₂SO₄)梯度中的浮力密度进行分离,这种梯度能解离非共价复合物。mRNA的交联也可用酚 - 氯仿抽提法进行检测。用蛋白酶K消化从交联复合物中回收的mRNA,其在聚丙烯酰胺凝胶中的电泳迁移率与未照射的mRNA相同。因此,照射既不会使RNA分子与RNA分子交联,也不会断裂磷酸二酯键。通过这些方法发现,超过70%的高分子量多分散mRNA能与蛋白质交联,但组蛋白mRNA只有25 - 40%能与蛋白质交联。基于浮力密度,组蛋白mRNA - 蛋白质复合物的蛋白质含量为26%,而大多数非组蛋白mRNA - 蛋白质复合物的平均蛋白质含量为65%。得出的结论是,多核糖体中的大多数mRNA与蛋白质紧密接触,并且组蛋白mRNA与蛋白质交联的数量比大多数其他mRNA少得多。

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