Brr2解旋U4/U6 SnRNAs的调控机制

前体mRNA(precursor messager RNA,pre-mRNA)剪接是去除内含子和将外显子彼此连接形成成熟mRNA的过程。剪接过程在一个呈动态变化的大核糖核蛋白(ribonucleoprotein, RNP)复合体,即剪接体催化作用下完成。DExD/H-box RNA解旋酶在剪接体组装、激活及解聚过程中都发挥着重要作用。Brr2(bad response to refrigeration 2)这种DExD/H-box RNA解旋酶是构成U5稳定的亚单位。Brr2含有两个串联解旋酶盒结构,在剪接体激活中负责U4/U6的解旋,还参与剪接体催化及解聚过程,因此Brr2在剪接过程中必需具备严格的调控机制。在剪接过程中,Prp8的C端包含两个连续的RNase H域和Jab1/MPN域,能够正负调控Brr2活性。Snu114在调节Brr2活性中具有非常重要的作用。此外,Brr2通过C端解旋酶盒(C-terminal cassette, CC)与N末端域(N-terminal region)进行分子内的自我活性调节。本文综述了近年来在Brr2的分子间和分子内活性调节机制的研究进展,这些不同的调节机制协同作用才确保真核生物pre-mRNA可变剪接的保真性。     

In vivo kinetics of U4/U6·U5 tri-snRNP formation in Cajal bodies

The U4/U6·U5 tri-small nuclear ribonucleoprotein particle (tri-snRNP) is an essential pre-mRNA splicing factor, which is assembled in a stepwise manner before each round of splicing. It was previously shown that the tri-snRNP is formed in Cajal bodies (CBs), but little is known about the dynamics of this process. Here we created a mathematical model of tri-snRNP assembly in CBs and used it to fit kinetics of individual snRNPs monitored by fluorescence recovery after photobleaching. A global fitting of all kinetic data determined key reaction constants of tri-snRNP assembly. Our model predicts that the rates of di-snRNP and tri-snRNP assemblies are similar and that ∼230 tri-snRNPs are assembled in one CB per minute. Our analysis further indicates that tri-snRNP assembly is approximately 10-fold faster in CBs than in the surrounding nucleoplasm, which is fully consistent with the importance of CBs for snRNP formation in rapidly developing biological systems. Finally, the model predicted binding between SART3 and a CB component. We tested this prediction by Förster resonance energy transfer and revealed an interaction between SART3 and coilin in CBs.     

神经介素U(neuromedin U)研究概况

神经介素 (ｎｅｕｒｏｍｅｄｉｎ)是一组平滑肌刺激性多肽 ,通常分成四类 :韩蛙皮素类、肛褶蛙肽类、神经紧张素类、神经介素Ｕ (ｎｅｒｕｏｍｅｄｉｎＵ ,ＮＭＵ) .在这组多肽中 ,神经介素Ｕ最后被发现 ,并因其子宫收缩活性而得名 .神经介素Ｕ是Ｍｉｎａｍｉｎｏ等在 1985年首次从猪脊髓中发现并分离提纯到的多肽 (包括ＮＭＵ 8和ＮＭＵ 2 5 ) ,随后又相继从大鼠、几内亚小猪、狗、家兔、鸡和澳大利亚树蛙等物种中分离得到 .ＮＭＵ产生于一个由 174个氨基酸组成的前体 .该前体包含一个疏水信号肽和几个二元蛋白酶加工位点 ,这些二元加工位…     

白血病耐药细胞系U937/ADR的建立及其生物学性状

目的：建立白血病耐药细胞系U937/ADR模型,并检测其多药耐药相关基因及其生物学性状的改变。方法：以大剂量阿霉素(IC50浓度),短时间(2h)暴露法诱导人白血病细胞系U937细胞的阿霉素耐药性。检测细胞的生长曲线,计算阿霉素耐药倍数,流式细胞术分析细胞周期分布;罗丹明123检测药物外排功能;荧光定量PCR（FQ-PCR）检测MDR1、MRP1、NF-Κb、Bcl-2、Bax mRNA水平变化;Western blot 检测Akt、p-Akt、P65、P-gp、MRP1和Bcl-2蛋白水平变化。结果：成功构建耐阿霉素U937/ADR细胞系,对阿霉素耐药指数为亲代U937细胞的11倍,U937/ADR群体倍增时间为43.6h,高于亲代细胞8.9h;流式细胞分析显示与U937细胞相比,U937/ADR的G0/G1期细胞增多,而G2/M期细胞减少。并对多种化疗药物产生交叉耐药性。罗丹明123外排试验显示,U937/ADR细胞外排明显增加。U937/ADR细胞MDR1、NF-Κb、Bcl-2 mRNA表达水平明显增加,P-gp及p-Akt、P65表达水平增加。结论：成功构建的U937/ADR细胞系其生物学特性明显不同与亲代U937细胞,对多种化疗药物产生多药耐药,高表达多药耐药蛋白P-gp,同时激活p-Akt及NF-Kb。     

U83 Box C/D snoRNA构建果蝇科系统发生树

利用已报道的黑腹果蝇U83基因搜索果蝇基因数据库,鉴定了10种新的果蝇科U83同源基因,它们均位于相应物种核蛋白基因rpl3的内含子中。以冈比亚按蚊为外类群,对11种果蝇的U83核苷酸序列作进化关系分析,用邻接法重建了系统发生树,结果与传统方法构建的系统发生树相比,能反映果蝇科的大致进化关系,但还存在部分差别。为增加序列信息,把序列长度拓展至整个U83所在的内含子,同法构建系统发生树,结果与传统系统发生树几乎完全一致。该研究是用boxC/D snoRNA基因序列构建系统发生树的首次尝试,实验结果证明U83可以很好地用于构建果蝇科内各物种的种系发生树。     

MEK1/2抑制剂U0126抑制肠道病毒71型的复制

为了揭示肠道病毒71型(enterovirus71,EV71)的复制与宿主细胞Raf/MEK/ERK信号通路(简称ERK通路)的相互关系,本研究应用临床诊断为手足口病的患儿疱疹液,通过易感细胞分离培养、RT-PCR及序列测定,以及Western印迹技术等方法,成功分离到EV71临床株.进一步用该分离株感染易感细胞,通过观察宿主细胞p-ERK1/2蛋白磷酸化水平、病毒特异性衣壳蛋白VP1水平、病毒半数组织培养感染量(50%tissue culture infectious dose,TCID50),以及感染细胞的CPE等指标,以期揭示ERK通路在EV71复制的作用.结果表明,EV71的复制可引起细胞ERK通路的活化;而用MEK1/2特异性的抑制剂U0126预先抑制ERK通路的活化,可显著地降低受染细胞上清液中的病毒的感染滴度(以TCID50表示)、受染细胞中EV71VP1蛋白水平、受染细胞中EV71核酸水平,以及受染细胞的细胞病变效应(cytopathic effect,CPE).提示ERK信号通路的活化对EV71的复制具有重要的作用.本研究为进一步阐明EV71在宿主细胞内的复制机制、寻找新型抗病毒靶标等研究奠定了良好的基础.     

A/U富集片段RNA结合蛋白的固相纯化与鉴定

RNA与细胞靶蛋白结合是RNA发挥其生物学功能的重要基础,因此,分离和鉴定RNA结合蛋白是研究RNA功能的必要步骤．目前,RNA结合蛋白的分离和鉴定方法较多,但各有优缺点．本实验利用可溶性碳二亚胺(EDC)介导的缩合反应,将A/U富集片段RNA共价偶联到固相介质amine M-270上,再用固定化RNA经亲和层析从细胞抽提物中分离纯化RNA结合蛋白,并以SDS-PAGE联合质谱分析和Western blotting等方法鉴定RNA特异性结合蛋白．最后通过荧光原位杂交和共聚焦显微镜证明这些RNA特异性结合蛋白确与RNA在细胞内结合．实践证明这一方法简单、高效、易于掌握．     

Endogenous U2·U5·U6 snRNA complexes in S. pombe are intron lariat spliceosomes

Excision of introns from pre-mRNAs is mediated by the spliceosome, a multi-megadalton complex consisting of U1, U2, U4/U6, and U5 snRNPs plus scores of associated proteins. Spliceosome assembly and disassembly are highly dynamic processes involving multiple stable intermediates. In this study, we utilized a split TAP-tag approach for large-scale purification of an abundant endogenous U2·U5·U6 complex from Schizosaccharomyces pombe. RNAseq revealed this complex to largely contain excised introns, indicating that it is primarily ILS (intron lariat spliceosome) complexes. These endogenous ILS complexes are remarkably resistant to both high-salt and nuclease digestion. Mass spectrometry analysis identified 68, 45, and 43 proteins in low-salt-, high-salt-, and micrococcal nuclease-treated preps, respectively. The protein content of a S. pombe ILS complex strongly resembles that previously reported for human spliced product (P) and Saccharomyces cerevisiae ILS complexes assembled on single pre-mRNAs in vitro. However, the ATP-dependent RNA helicase Brr2 was either substoichiometric in low-salt preps or completely absent from high-salt and MNase preps. Because Brr2 facilitates spliceosome disassembly, its relative absence may explain why the ILS complex accumulates logarithmically growing cultures and the inability of S. pombe extracts to support in vitro splicing.     

Sfrp2通过下调Wnt/β-catenin通路抑制胶质瘤细胞系U251的迁移能力

摘要 目的：探讨使用Wnt3a蛋白受体竞争性抑制剂Sfrp2下调Wnt通路的关键蛋白β-catenin的表达对胶质瘤细胞U251线粒体功能以及细胞侵袭能力的影响。方法：使用外源性Sfrp2蛋白处理U251细胞,使用Western Blot技术,Mitotracker线粒体形态学染色,划痕实验观测Sfrp2蛋白对U251细胞Wnt通路的表达,线粒体功能以及细胞迁移能力的影响,并使用GSK-3β抑制剂LiCl上调Wnt通路进一步明确Sfrp2蛋白的作用机制。结果：Sfrp2蛋白可引起Wnt通路的抑制（P<0.05）,线粒体分裂（P<0.01）以及细胞迁移能力的下降（P<0.01）,而使用LiCl处理后,Wnt通路重现上调（P<0.05）,线粒体分裂受到抑制（P<0.05）,细胞的迁移能力也再次恢复（P<0.05）。结论：Sfrp2可通过下调Wnt通路引起线粒体分裂进而抑制U251细胞的迁移能力。     

Characterization of autoantibodies that recognize U4/U6 small ribonucleoprotein particles in serum from a patient with primary Sj?gren's syndrome.

We identified autoantibodies that recognize the U4/U6 snRNPs in a serum from a 63-year-old Japanese patient (TT) with primary Sj?gren's syndrome. This patient's serum immunoprecipitated U4 and U6 sn-RNAs exclusively from 32P-labeled HeLa cell extracts and a newly identified 120-kDa protein along with the Sm core proteins (B'/B, D, E, F, and G) from [35S] methionine-labeled HeLa cell extracts. Immunoblotting demonstrated that only the 120-kDa protein was recognized by this unique serum. In glycerol density gradient centrifugation, the 120-kDa protein reactive with TT serum cosedimented with U4 and U6 snRNAs, suggesting that the 120-kDa protein is a unique component of the U4/U6 snRNP particle. In the same study, the U4/U6 snRNP precipitated by TT serum sedimented only in the lower density, whereas anti-Sm antibodies precipitated U4/U6 snRNAs in a broad range of the gradient. This result suggests the presence of at least two molecular forms of the U4/U6 snRNP particles; larger particles, probably the U4/U5/U6 snRNP complex, and free particles. Thus, the U4/U6 snRNP recognized by TT serum includes the U4 and U6 snRNAs, with Sm core proteins, and the novel 120-kDa protein, and appears to be a free particle not associated with larger complexes.     

黑曲霉(Aspergillus niger) Uγ-2菊粉酶保护剂的研究*

研究菊粉酶热稳定性,菊粉酶在60℃具有较好的热稳定性;一些醇类物质和增稠剂可以提高菊粉酶的热稳定性;利用甘油、黄原胶和CaCl₂设计三因素三水平的正交试验,确定了以6%的甘油,0·6%的黄原胶,100mmol/L的CaCl₂组合的保护剂,对提高酶的热稳定性具有显著作用。     

超微粒TiO2对U937细胞光杀伤效应及机理研究

超微粒TiO₂经光催化氧化后对U937白血病细胞有明显的杀伤作用,DNA琼脂糖凝胶电泳图证明了光激发TiO₂能够损伤细胞内的DNA,从而导致细胞死亡,提出了一种杀伤癌细胞的新思路.