Skålhegg B S, Landmark B, Foss K B, Lohmann S M, Hansson V, Lea T, Jahnsen T
Institute of Pathology, Rikshospitalet, Oslo, Norway.
J Biol Chem. 1992 Mar 15;267(8):5374-9.
We have previously identified and characterized regulatory (R) subunits of cyclic AMP-dependent protein kinase, particularly the RII subunits in rat tissues (Jahnsen, T., Lohmann, S. M., Walter, U., Hedin, L., and Richards, J. S. (1985) J. Biol. Chem. 260, 15980-15987; Jahnsen, T., Hedin, L., Lohmann, S. M., Walter, U., and Richards, J. S. (1986) J. Biol. Chem. 261, 6637-6639; Jahnsen, T., Hedin, L., Kidd, V. J., Beattie, W. G., Lohmann, S. M., Walter, U., Durica, J., Schulz, T. Z., Schiltz, E., Browner, M., Lawrence, C. B., Goldman, D., Ratoosh, S. L., and Richards, J. S. (1986) J. Biol. Chem. 261, 12352-12361). These studies showed that rat RII alpha and RII beta had apparent molecular masses of 54 and 52 kDa, respectively. The aim of the present study was to purify and characterize cAMP-dependent protein kinase R subunits in human testis and to examine which of the subunits (mRNAs and proteins) are present in this tissue. Our results show that human testis contains mRNAs for five out of the seven known subunits of cAMP-dependent protein kinase. We observed strong expression of mRNAs for RI alpha (1.5 and 3.2 kilobases (kb)), RII alpha (2.2, 2.4, and 7.0 kb), and RII beta (3.3 kb). We also demonstrated mRNAs for two of the three catalytic subunits, C alpha (2.7 kb) and C gamma (1.7 kb). Purification of R subunits by DEAE-cellulose and cAMP affinity chromatography revealed three distinct forms with apparent molecular masses of 49, 51, and 53 kDa, respectively. Characterization of these R subunits by their 8-azido-cAMP photoaffinity labeling and immunoreactivity, as well as by a phosphorylation-dependent mobility shift on sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE), indicated subunit sizes of RII beta (53 kDa) greater than RII alpha dephosphoform (51 kDa) greater than RI alpha (49 kDa). This conclusion was verified by the analysis of RII subunits produced by in vitro transcription/translation of full-length cDNAs for both human RII alpha and RII beta in wheat germ lysates. The in vitro translated products were the same size as the purified human testis subunits, and only the smallest RII subunit (RII alpha) revealed a distinct mobility shift on SDS-PAGE after phosphorylation/dephosphorylation. This study supports the conclusion that the mobilities of human RII subunits (RII alpha, RII beta) on SDS-PAGE are reversed in contrast with those of other species such as rat and bovine.(ABSTRACT TRUNCATED AT 400 WORDS)
我们之前已经鉴定并表征了环磷酸腺苷(cAMP)依赖性蛋白激酶的调节(R)亚基,特别是大鼠组织中的RII亚基(扬森,T.,洛曼,S.M.,瓦尔特,U.,赫丁,L.,以及理查兹,J.S.(1985年)《生物化学杂志》260,15980 - 15987;扬森,T.,赫丁,L.,洛曼,S.M.,瓦尔特,U.,以及理查兹,J.S.(1986年)《生物化学杂志》261,6637 - 6639;扬森,T.,赫丁,L.,基德,V.J.,贝蒂,W.G.,洛曼,S.M.,瓦尔特,U.,杜里卡,J.,舒尔茨,T.Z.,席尔茨,E.,布朗纳,M.,劳伦斯,C.B.,戈德曼,D.,拉托什,S.L.,以及理查兹,J.S.(1986年)《生物化学杂志》261,12352 - 12361)。这些研究表明,大鼠的RIIα和RIIβ的表观分子量分别为54 kDa和52 kDa。本研究的目的是纯化并表征人类睾丸中的cAMP依赖性蛋白激酶R亚基,并检测该组织中存在哪些亚基(mRNA和蛋白质)。我们的结果表明,人类睾丸中含有cAMP依赖性蛋白激酶七个已知亚基中的五个的mRNA。我们观察到RIα(1.5和3.2千碱基(kb))、RIIα(2.2、2.4和7.0 kb)以及RIIβ(3.3 kb)的mRNA有强烈表达。我们还证实了三个催化亚基中的两个,即Cα(2.7 kb)和Cγ(1.7 kb)的mRNA的存在。通过DEAE - 纤维素和cAMP亲和层析纯化R亚基,得到了三种不同形式,其表观分子量分别为49 kDa、51 kDa和53 kDa。通过它们的8 - 叠氮基 - cAMP光亲和标记和免疫反应性,以及在十二烷基硫酸钠 - 聚丙烯酰胺凝胶电泳(SDS - PAGE)上的磷酸化依赖性迁移率变化对这些R亚基进行表征,结果表明亚基大小顺序为RIIβ(53 kDa)大于RIIα去磷酸化形式(51 kDa)大于RIα(49 kDa)。通过对在小麦胚芽裂解物中对人类RIIα和RIIβ的全长cDNA进行体外转录/翻译所产生的RII亚基的分析,验证了这一结论。体外翻译产物与纯化的人类睾丸亚基大小相同,并且只有最小的RII亚基(RIIα)在磷酸化/去磷酸化后在SDS - PAGE上显示出明显的迁移率变化。本研究支持这样的结论,即与大鼠和牛等其他物种相比,人类RII亚基(RIIα、RIIβ)在SDS - PAGE上的迁移率是相反的。(摘要截断于400字)
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