Burch W M, Lebovitz H E
J Clin Invest. 1980 Sep;66(3):532-42. doi: 10.1172/JCI109885.
We used embryonic chick pelvic cartilage as a model to study the mechanism by which cyclic AMP increases RNA synthesis. Isolated nuclei were incubated with [32P]-8-azidoadenosine 3,5'-monophosphate ([32P]N3cAMP) with no resultant specific nuclear binding. However, in the presence of cytosol proteins, nuclear binding of [32P]N3cAMP was demonstrable that was specific, time dependent, and dependent on a heat-labile cytosol factor. The possible biological significance of the nuclear binding of the cyclic AMP-protein complex was identified by incubating isolating nuclei with either cyclic AMP or cytosol cyclic AMP-binding proteins prepared by batch elution DEAE cellulose chromatography (DEAE peak cytosol protein), or both, in the presence of cold nucleotides and [3H]uridine 5'-triphosphate. Poly(A) RNA production occurred only in nuclei incubated with cyclic AMP and the DEAE peak cytosol protein preparation. Actinomycin D inhibited the incorporation of [3H]uridine 5'-monophosphate into poly(A) RNA. The newly synthesized poly(A) RNA had a sedimentation constant of 23S. Characterization of the cytosol cyclic AMP binding proteins using [32P]N3-cAMP with photoaffinity labeling three major cAMP-binding complexes (41,000, 51,000, and 55,000 daltons). The 51,000 and 55,000 dalton cyclic AMP binding proteins were further purified by DNA-cellulose chromatography. In the presence of cyclic AMP they stimulated poly(A) RNA synthesis in isolated nuclei. The 51,000-dalton cyclic AMP-binding protein was the predominant one that bound to the nuclei. While cyclic AMP-dependent protein kinsae activity was present in the cytosol and DEAE peak cytosol proteins, it was not present in the DNA-cellulose-bound, cyclic AMP-binding proteins. We conclude that one possible mechanism by which cyclic AMP increases RNA synthesis is by complexing to a 51,000-dalton cytosol cyclic AMP-binding protein and being subsequently translocated to the nucleus, where it is specifically bound and associated with induction of poly(A) RNA synthesis.
我们以鸡胚骨盆软骨为模型,研究环磷酸腺苷(cAMP)增加RNA合成的机制。将分离的细胞核与[32P]-8-叠氮腺苷3,5'-单磷酸([32P]N3cAMP)一起孵育,未产生特异性核结合。然而,在存在胞质溶胶蛋白的情况下,[32P]N3cAMP的核结合是可证明的,这种结合具有特异性、时间依赖性,并且依赖于一种热不稳定的胞质溶胶因子。通过在冷核苷酸和[3H]尿苷5'-三磷酸存在的情况下,将分离的细胞核与cAMP或通过分批洗脱DEAE纤维素色谱法制备的胞质溶胶cAMP结合蛋白(DEAE峰胞质溶胶蛋白)或两者一起孵育,确定了cAMP-蛋白复合物核结合的可能生物学意义。只有在与cAMP和DEAE峰胞质溶胶蛋白制剂一起孵育的细胞核中才会发生聚腺苷酸(Poly(A))RNA的产生。放线菌素D抑制[3H]尿苷5'-单磷酸掺入聚腺苷酸(Poly(A))RNA中。新合成的聚腺苷酸(Poly(A))RNA的沉降常数为23S。使用[32P]N3-cAMP进行光亲和标记对胞质溶胶cAMP结合蛋白进行表征,发现了三种主要的cAMP结合复合物(41,000、51,000和55,000道尔顿)。51,000和55,000道尔顿的cAMP结合蛋白通过DNA纤维素色谱法进一步纯化。在cAMP存在的情况下,它们刺激分离细胞核中的聚腺苷酸(Poly(A))RNA合成。51,000道尔顿的cAMP结合蛋白是与细胞核结合的主要蛋白。虽然cAMP依赖性蛋白激酶活性存在于胞质溶胶和DEAE峰胞质溶胶蛋白中,但不存在于DNA纤维素结合的cAMP结合蛋白中。我们得出结论,cAMP增加RNA合成的一种可能机制是与一种51,000道尔顿的胞质溶胶cAMP结合蛋白形成复合物,随后转移到细胞核中,在那里它被特异性结合并与聚腺苷酸(Poly(A))RNA合成的诱导相关。
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