黑曲霉pepB基因缺失菌株的构建及其功能分析

以黑曲霉(Aspergillus niger)GICC2773基因组DNA为模板,用PCR方法分别扩增pepB基因中的上游约1．4kb和下游约1．3kb两段DNA序列,将此两段序列按同一方向分别插入质粒pMW1中潮霉素抗性基因(hph)表达单元的5′和3′端,构建成重组质粒pMW1-pepB,用于通过同源重组靶向破坏基因组中的pepB基因。同源重组则采用原生质体-PEG方法,将酶切pMW1-pepB得到的线性片段转化A．niger GICC2773菌株,通过潮霉素选择平板得到62个Hgy抗性转化子,然后采用PCR方法从这些抗性转化子中筛选到1个由于同源重组产生的pepB基因缺失突变菌株pepB29。功能分析显示该突变株的酸性蛋白酶活性有明显下降,外源蛋白漆酶的分泌表达有所提高。     

同源重组法制备口蹄疫病毒多基因重组腺病毒

通过细菌内同源重组的方法成功构建了含有O型口蹄疫病毒P1—2A和3C蛋白酶基因和3D基因的重组腺病毒表达载体。首先将P1—2A、3C和3D基因亚克隆连接到穿梭质粒pShuttle—CMV上,再将重组穿梭质粒用PmeI线性化后电转化携带有腺病毒骨架载体pAdeasy—1的大肠杆菌BJ5183感受态菌,经细菌内同源重组产生pAdcmv—p12x3c和pAdcmy—p12x3cd重组腺病毒质粒,经序列测定证实目的基因已正确的插入到腺病毒骨架载体中。重组腺病毒质粒经PacI线性化后转染HEK293细胞,转染1w内细胞出现典型病变。取转染细胞裂解液上清连续传代至第4代时,细胞于24～48h内即病变完全,收取接毒后24h细胞进行。PCR和RT—PCR检测,表明目的基因已整合到腺病毒基因组内,且在mRNA水平上有表达。取第4、6、8和10代病毒,用蛋白酶K处理后可扩增出目的基因,证明此重组病毒可稳定存在。本研究为FMDV腺病毒活载体疫苗的研究奠定了基础。     

Nuclear localization of Rad52 is pre-requisite for its sumoylation

In Saccharomyces cerevisiae, Rad52 plays major roles in several types of homologous recombination. Here, we found that rad52-K200R mutation greatly reduced sumoylation of Rad52. The rad52-K200R mutant exhibited defects in various types of recombination, such as intrachromosomal recombination and mating-type switching. The K200 residue of Rad52 is part of the nuclear localization signal (NLS), which is important for transport into the nucleus. Indeed, the addition of a SV40 NLS to Rad52-K200R suppressed the sumoylation defect of Rad52-K200R. These findings indicate that nuclear localization of Rad52 is pre-requisite for its sumoylation.     

MAD2蛋白在蚕豆细胞周期中的同源定位

细胞周期是一个高度有序的过程,其运行过程受到多个检验点(checkpoint)的严格监控.MAD2是动物细胞纺锤体检验点(spindle checkpoint)中一种重要的蛋白。我们利用免疫印记法从蚕豆组织中检测到一种MAD2的同源蛋白,该蛋白的分子量在26KD左右,其亚细胞分布方式与动物细胞大致相同,都随细胞周期的进行而变化:在间期细胞中,MAD2分布于整个细胞中,并且在核膜外侧有优先聚集;在有丝分裂前期细胞中,MAD2在核膜破裂后开始在动粒处聚集;到早中期(prometaphase),MAD2定位于动粒;随着微管的延伸,MAD2逐渐减少直至消失,在中期,晚中期及后期细胞中,动粒处已无MAD2的分布。     

桑树二倍体及人工诱导的同源四倍体遗传差异的AFLP分析

利用AFLP(AmplifiedFragmentLengthPolymorphism)分子标记技术 ,即扩增片段长度多态性 ,从DNA分子水平探讨二倍体桑 (2n =2X =2 8)与经秋水仙素诱变得到的同源四倍体桑 (2n =4X =5 6 )在遗传结构上的差异。根据对供试材料DNA多态性及遗传距离分析 ,认为经秋水仙素诱变得到的同源 4X与 2X相比在DNA分子遗传结构上产生一定程度的改变 ,在种内变异水平上 ,2X与同源 4X桑间的遗传差异小于种间差异。     

Production of recombinant granulocyte colony-stimulating factor by knocking into the active immunoglobulin heavy chain gene locus in the hybridoma cell line

The hybridoma cell line KM50 originally produces a monoclonal antibody at a concentration of ∼40 mg ml^-1 in ascites. To investigate the possibility to apply this expression system to the production of useful proteins, the cDNA encoding human granulocyte colony-stimulating factor was inserted by homologous recombination into just downstream of the promoter of the active immunoglobulin heavy chain gene of KM50. Site directed integration of targeting DNAs resulted in the disruption of expression of the immunoglobulin heavy chain proteins with a frequency of 1 in 10 ∼ 100 G418-resistance transfectants. One of the monoclonal antibody-deficient transfectants produced25 ng ml^-1 of granulocyte colony-stimulating factor in the supernatant of its cell culture the number of molecules of which corresponds to that of the monoclonal antibody originally produced by KM50. However, when this transfectant was injected intraperitoneally, it produced only a 9 μg ml^-1 concentration of granulocyte colony-stimulating factor in ascites, which is approximately 3 orders of magnitude less than the monoclonal antibody. This method may be applicable to production of other recombinant proteins, although further optimization in the conditions of production would be needed in order to reach much higher yields. This revised version was published online in August 2006 with corrections to the Cover Date.     

Extending the Horizon of Homology Detection with Coevolution-based Structure Prediction

Traditional sequence analysis algorithms fail to identify distant homologies when they lie beyond a detection horizon. In this review, we discuss how co-evolution-based contact and distance prediction methods are pushing back this homology detection horizon, thereby yielding new functional insights and experimentally testable hypotheses. Based on correlated substitutions, these methods divine three-dimensional constraints among amino acids in protein sequences that were previously devoid of all annotated domains and repeats. The new algorithms discern hidden structure in an otherwise featureless sequence landscape. Their revelatory impact promises to be as profound as the use, by archaeologists, of ground-penetrating radar to discern long-hidden, subterranean structures. As examples of this, we describe how triplicated structures reflecting longin domains in MON1A-like proteins, or UVR-like repeats in DISC1, emerge from their predicted contact and distance maps. These methods also help to resolve structures that do not conform to a “beads-on-a-string” model of protein domains. In one such example, we describe CFAP298 whose ubiquitin-like domain was previously challenging to perceive owing to a large sequence insertion within it. More generally, the new algorithms permit an easier appreciation of domain families and folds whose evolution involved structural insertion or rearrangement. As we exemplify with α1-antitrypsin, coevolution-based predicted contacts may also yield insights into protein dynamics and conformational change. This new combination of structure prediction (using innovative co-evolution based methods) and homology inference (using more traditional sequence analysis approaches) shows great promise for bringing into view a sea of evolutionary relationships that had hitherto lain far beyond the horizon of homology detection.     

The Caenorhabditis elegansRAD51 homolog is transcribed into two alternative mRNAs potentially encoding proteins of different sizes

In prokaryotes, the RecA protein plays a pivotal role in homologous recombination, catalyzing the transfer of a single DNA strand into an homologous molecule. Structural homologs of the bacterial RecA protein, called Rad51, have been found in different eukaryotes (from yeast to man), suggesting a certain level of conservation in recombination pathways among living organisms. We have cloned the homolog of RAD51 in Caenorhabditis elegans. The CeRAD51 gene is transcribed into two alternative mRNAs and potentially codes for two proteins of 395 and 357 amino acids in length, respectively. We discuss the evolutionary implications of these findings. Received: 26 May 1998 / Accepted: 18 August 1998