Delaney Kimberly J, Xu Ruqiang, Zhang Jingxian, Li Q Quinn, Yun Kil-Young, Falcone Deane L, Hunt Arthur G
Department of Plant and Soil Sciences, University of Kentucky, Lexington, Kentucky 40546-0312, USA.
Plant Physiol. 2006 Apr;140(4):1507-21. doi: 10.1104/pp.105.070672. Epub 2006 Feb 24.
The Arabidopsis (Arabidopsis thaliana) gene that encodes the probable ortholog of the 30-kD subunit of the mammalian cleavage and polyadenylation specificity factor (CPSF) is a complex one, encoding small (approximately 28 kD) and large (approximately 68 kD) polypeptides. The small polypeptide (AtCPSF30) corresponds to CPSF30 and is the focus of this study. Recombinant AtCPSF30 was purified from Escherichia coli and found to possess RNA-binding activity. Mutational analysis indicated that an evolutionarily conserved central core of AtCPSF30 is involved in RNA binding, but that RNA binding also requires a short sequence adjacent to the N terminus of the central core. AtCPSF30 was found to bind calmodulin, and calmodulin inhibited the RNA-binding activity of the protein in a calcium-dependent manner. Mutational analysis showed that a small part of the protein, again adjacent to the N terminus of the conserved core, is responsible for calmodulin binding; point mutations in this region abolished both binding to and inhibition of RNA binding by calmodulin. Interestingly, AtCPSF30 was capable of self-interactions. This property also mapped to the central conserved core of the protein. However, calmodulin had no discernible effect on the self-association. These results show that the central portion of AtCPSF30 is involved in a number of important functions, and they raise interesting possibilities for both the interplay between splicing and polyadenylation and the regulation of these processes by stimuli that act through calmodulin.
拟南芥(Arabidopsis thaliana)中编码哺乳动物切割与聚腺苷酸化特异性因子(CPSF)30-kD亚基可能直系同源物的基因结构复杂,可编码小(约28 kD)、大(约68 kD)两种多肽。小多肽(AtCPSF30)对应于CPSF30,是本研究的重点。重组AtCPSF30从大肠杆菌中纯化得到,具有RNA结合活性。突变分析表明,AtCPSF30进化上保守的中央核心区域参与RNA结合,但RNA结合还需要中央核心区域N端附近的一段短序列。发现AtCPSF30可结合钙调蛋白,且钙调蛋白以钙依赖的方式抑制该蛋白的RNA结合活性。突变分析显示,该蛋白中同样位于保守核心区域N端附近的一小部分负责与钙调蛋白结合;该区域的点突变消除了与钙调蛋白的结合以及对RNA结合的抑制作用。有趣的是,AtCPSF30能够自我相互作用。这一特性也定位于该蛋白的中央保守核心区域。然而,钙调蛋白对自我缔合没有明显影响。这些结果表明,AtCPSF30的中央部分参与多种重要功能,这为剪接与聚腺苷酸化之间的相互作用以及通过钙调蛋白起作用的刺激对这些过程的调控带来了有趣的可能性。