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Structural insights into the assembly of the 30S ribosomal subunit in vivo: functional role of S5 and location of the 17S rRNA precursor sequence
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作者 Zhixiu Yang Qiang Guo +9 位作者 Simon Goto Yuling Chen Ningning Li Kaige Yan Yixiao Zhang Akira Muto Haiteng Deng Hyouta Himeno Jianlin Lei Ning Gao 《Protein & Cell》 SCIE CAS CSCD 2014年第5期394-407,共14页
The in vivo assembly of ribosomal subunits is a highly complex process, with a tight coordination between protein assembly and rRNA maturation events, such as folding and processing of rRNA precursors, as well as modi... The in vivo assembly of ribosomal subunits is a highly complex process, with a tight coordination between protein assembly and rRNA maturation events, such as folding and processing of rRNA precursors, as well as modifications of selected bases. In the cell, a large number of factors are required to ensure the efficiency and fidelity of subunit production. Here we characterize the immature 30S subunits accumulated in a factor-null Escherichia coil strain (ArsgAArbfA). The immature 30S subunits isolated with varying salt concentrations in the buffer system show interesting differences on both protein composition and structure. Specifically, inter- mediates derived under the two contrasting salt condi- tions (high and low) likely reflect two distinctive assembly stages, the relatively early and late stages of the 3' domain assembly, respectively. Detailed structural analysis demonstrates a mechanistic coupling between the maturation of the 5' end of the 17S rRNA and the assembly of the 30S head domain, and attributes a unique role of S5 in coordinating these two events. Furthermore, our structural results likely reveal thelocation of the unprocessed terminal sequences of the 17S rRNA, and suggest that the maturation events of the 17S rRNA could be employed as quality control mech- anisms on subunit production and protein translation. 展开更多
关键词 RsgA rbfa ribosome assembly cryo-EM quantitative mass spectrometry
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骨关节病关节软骨中Cbfal含量的测定及其意义
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作者 蔡郑东 贾金鹏 +4 位作者 纪方 孙庆斌 张军 杨家荟 沈茜 《中国骨肿瘤骨病》 2003年第1期48-50,共3页
目的 通过定量检测骨关节病标本中核心结合因子al(Cbfal)含量的变化,探讨Cbfal在骨关节病中可能的作用机制。方法 采用实时荧光定量PCR的方法,定量检测15例髋关节骨关节病及4例膝关节骨关节病标本中损伤软骨与正常软骨Cbfal mRNA的含量... 目的 通过定量检测骨关节病标本中核心结合因子al(Cbfal)含量的变化,探讨Cbfal在骨关节病中可能的作用机制。方法 采用实时荧光定量PCR的方法,定量检测15例髋关节骨关节病及4例膝关节骨关节病标本中损伤软骨与正常软骨Cbfal mRNA的含量。结果 损伤软骨Cbfal mRNA的转录水平较正常软骨升高约38倍。结论 Cbfal在受损软骨部位表达,与骨关节病的发生过程有关,并可能是关节软骨部位钙化的重要原因之一。 展开更多
关键词 骨关节病 关节软骨细胞 测定 rbfa1含量
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