Expression and location of Smad2,4 mRNAs during and after liver fibrogenesis of rats

瞄准：在老鼠在肝调查 Smad2 和 Smad4 mRNAs 的地点改变在期间并且在纤维发生以后。方法：各称约 200 g 的八十只男 Wistar 老鼠被使用。试验性的肝的纤维变性的老鼠模型被注射与四氯化碳(CCl4 ) 建立，正常老鼠和老鼠与齐墩果油被注射并且担任了控制组。原位杂交(ISH ) 被用来在肝检测 Smad2 和 Smad4 mRNA。结果：原位杂交显示出 Smad2 和 Smad4 mRNA 在中央静脉和肝的湾穴在期间并且在纤维发生以后附近的在肝的星形细胞(HSC ) 的细胞质的表情，成纤维细胞和 myofibroblasts。Smad2 的表示， 4 mRNA 在正常和控制老鼠比那高。结论：在这个过程并且在肝的纤维变性形成， HSC，成纤维细胞和 myofibroblasts 以后是表示 Smad2 和 Smad4 的主要房间。肝的纤维变性在受伤的肝越严肃， Smad2 的水平和 Smad4 基因表示分别地是越多 higher 在期间并且在纤维发生以后。

Structural insights into the assembly of the 30S ribosomal subunit in vivo： functional role of S5 and location of the 17S rRNA precursor sequence

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.