利用果蝇模型研究人类心脏早期发育的分子机理(英文)

近年来 ,果蝇心脏特化的遗传机制已初步研究清楚 ,但控制人类心脏早期发育的基因尚待鉴定。因为调控果蝇和脊椎动物早期心脏细胞命运定型的途径具有保守性 ,果蝇是一种探讨人类心脏早期发育的分子机理的理想动物模式。为此目的 ,我们采用P转座子和EMS诱变技术建立了约 3 0 0 0个隐性致死基因平衡系。通过心脏前体细胞特异性抗体免疫组化筛选 ,我们检出 2 0 0余个表现心脏突变表型的平衡致死系。我们进一步利用RNAi技术对一些基因的功能进行了初步的研究 ,证明这些基因表现RNAi的突变表型 ,该类突变表型与基因突变时表现的表型相似 ,即心管呈缺陷型或无心脏前体细胞形成。利用果蝇和人类基因组计划获得的成果 ,我们从果蝇心脏侯选基因中初步克隆和鉴定了 5 0个人类同源基因 ,其中 2 0个是新基因。Northen印迹分析表明 ,一部分人类基因在心脏组织中有表达 ,从而为研究这些基因在人类心脏早期发育中的作用提供了信息。目前 ,我们正在建立转基因果蝇 ,以此为模型研究这些基因是否对心肌细胞发生或心肌功能起调控作用。产生心肌细胞突变类型的基因如果类似于人类心脏病综合症 ,则可以作为人类心脏疾病侯选基因作进一步的分析。     

酵母双杂交技术筛选hCLP46的相互作用蛋白

目的:利用酵母双杂交技术,筛选人白细胞cDNA文库中能与人类CD34 干/祖细胞异常表达蛋白hCLP46(human CAP10-like protein46)相互作用的未知蛋白.通过对其相互作用蛋白的筛选和研究,研究hCLP46基因在骨髓增生异常综合症MDS-AML的作用机制.为MDS-AML的临床治疗和诊断提供理论基础.方法:以pGBKT7-hCLP46为诱饵质粒筛选人白细胞cDNA文库,得到阳性克隆,并对验证后的阳性克隆的外源性片段进行测序及同源性分析.结果:经过两次筛选、验证,从人白细胞cDNA文库中得到5个阳性克隆,对验证后的阳性克隆的外源片段进行测序及同源性分析,最终得到4个不同的候选基因序列.结论:应用酵母双杂交系统,共筛选得到4个不同的基因,其编码蛋白与hCLP46有相互作用,可能与MDS-AML发病机制相关.     

肝细胞生成素在睾丸组织中的相互作用蛋白

肝细胞生成素（HPO）具有复杂的生理功能,在睾丸中的高表达提示其在生殖活动中的重要性,而不仅局限于肝再生.构建了酵母表达载体pGBKT7-HPO,采用酵母双杂交系统,以HPO为诱饵蛋白,从人睾丸cDNA文库中寻找能够与HPO相互作用的蛋白质.经过筛选、验证阳性克隆,并进行PCR、测序和序列比对,得到4种相互作用蛋白质：NADH脱氢酶1、钠/钾ATP酶β3亚基、磷脂酶C δ1以及附睾分泌蛋白.提示HPO可能参与了细胞的蛋白质合成,能量代谢等.通过对候选蛋白的研究,为探讨HPO对睾丸组织细胞功能的调节机制提供了重要的线索.     

Micromanipulator for Yeast Genetic Studies

An inexpensive mechanical micromanipulator, designed primarily for separating yeast ascospores, can be assembled from commercially available components and without extensive custom machining.     

利用酵母双杂交技术筛选与AtbZIP1相互作用的蛋白质

碱性亮氨酸拉链bZIP类转录因子在植物的生长发育、光形态建成、光信号传导及非生物胁迫反应中发挥重要的作用.为研究AtbZIP1基因的作用机理,本研究首先验证了该基因的自激活转录活性,通过缺失突变确定了该转录因子的转录激活结构域;以AtbZIP1缺失突变体AtbZ3为诱饵蛋白,采用Matchmaker Gold Yeast Two-Hybrid System(Clonetch),共筛选获得5个与诱饵蛋白相互作用的蛋白质;并通过AbA(Aureobasidin A)抗生素标记基因,His营养缺陷和LacZ蓝白斑检测验证了阳性克隆.亚细胞定位分析发现,AtbZIP1蛋白除了定位于细胞核外,还定位于叶绿体细胞.通过分析这些靶蛋白的已知功能,为研究AtbZIP1蛋白的未知生物学功能提供重要信息.     

Comparison of Methods for Separating Proteins Using Bisalbuminemia as a Model

Sera from bisalbuminemic chicken-turkey hybrids contain two albumins in equal amounts. These are observed as inherited electrophoretic variants and originate from the respective chicken and turkey parents. Sera from the hybrid birds served as a model system by which fractionating and identification procedures for evaluating serum albumin variants were compared.

The two albumins in the hybrid were isolated with preparative polyacrylamide gel electrophoresis (PAGE) and starch block preparative electrophoresis. Isoelectric focusing of the hybrid albumins resulted in the isolation of the turkey albumin. Interference of ampholinea prevented the complete isolation of the chicken albumin.

The two albumins in the hybrid have identical molecular weights and cannot be identified by sedimentation coefficient, gel filtration behavior, or sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE). Because of the close relatedness the chicken and turkey albumins in the hybrid cross reacted with rabbit anti-hybrid serum as well as with rabbit anti-chicken and anti-turkey sera.     

Mapping the Interactions of Dengue Virus NS1 Protein with Human Liver Proteins Using a Yeast Two-Hybrid System: Identification of C1q as an Interacting Partner

Dengue constitutes a global health concern. The clinical manifestation of this disease varies from mild febrile illness to severe hemorrhage and/or fatal hypovolemic shock. Flavivirus nonstructural protein 1 (NS1) is a secreted glycoprotein that is displayed on the surface of infected cells but is absent in viral particles. NS1 accumulates at high levels in the plasma of dengue virus (DENV)-infected patients, and previous reports highlight its involvement in immune evasion, dengue severity, liver dysfunction and pathogenesis. In the present study, we performed a yeast two-hybrid screen to search for DENV2 NS1-interacting partners using a human liver cDNA library. We identified fifty genes, including human complement component 1 (C1q), which was confirmed by coimmunoprecipitation, ELISA and immunofluorescence assays, revealing for the first time the direct binding of this protein to NS1. Furthermore, the majority of the identified genes encode proteins that are secreted into the plasma of patients, and most of these proteins are classified as acute-phase proteins (APPs), such as plasminogen, haptoglobin, hemopexin, α-2-HS-glycoprotein, retinol binding protein 4, transferrin, and C4. The results presented here confirm the direct interaction of DENV NS1 with a key protein of the complement system and suggest a role for this complement protein in the pathogenesis of DENV infection.     

Mismatch Repair Proteins Regulate Heteroduplex Formation during Mitotic Recombination in Yeast

Mismatch repair (MMR) proteins actively inhibit recombination between diverged sequences in both prokaryotes and eukaryotes. Although the molecular basis of the antirecombination activity exerted by MMR proteins is unclear, it presumably involves the recognition of mismatches present in heteroduplex recombination intermediates. This recognition could be exerted during the initial stage of strand exchange, during the extension of heteroduplex DNA, or during the resolution of recombination intermediates. We previously used an assay system based on 350-bp inverted-repeat substrates to demonstrate that MMR proteins strongly inhibit mitotic recombination between diverged sequences in Saccharomyces cerevisiae. The assay system detects only those events that reverse the orientation of the region between the recombination substrates, which can occur as a result of either intrachromatid crossover or sister chromatid conversion. In the present study we sequenced the products of mitotic recombination between 94%-identical substrates in order to map gene conversion tracts in wild-type versus MMR-defective yeast strains. The sequence data indicate that (i) most recombination occurs via sister chromatid conversion and (ii) gene conversion tracts in an MMR-defective strain are significantly longer than those in an isogenic wild-type strain. The shortening of conversion tracts observed in a wild-type strain relative to an MMR-defective strain suggests that at least part of the antirecombination activity of MMR proteins derives from the blockage of heteroduplex extension in the presence of mismatches.     

In-Cell Protease Assay Systems Based on Trans-Localizing Molecular Beacon Proteins Using HCV Protease as a Model System

This study describes a sensitive in-cell protease detection system that enables direct fluorescence detection of a target protease and its inhibition inside living cells. This live-cell imaging system provides a fluorescent molecular beacon protein comprised of an intracellular translocation signal sequence, a protease-specific cleavage sequence, and a fluorescent tag sequence(s). The molecular beacon protein is designed to change its intracellular localization upon cleavage by a target protease, i.e., from the cytosol to a subcellular organelle or from a subcellular organelle to the cytosol. Protease activity can be monitored at the single cell level, and accordingly the entire cell population expressing the protease can be accurately enumerated. The clear cellular change in fluorescence pattern makes this system an ideal tool for various life science and drug discovery research, including high throughput and high content screening applications.     

Hawaii as a Model System for Human Ecodynamics

The human ecodynamics approach in archaeology privileges landscape as a core concept, asserting that there can be no environment or ecosystem detached from humans and their behavior. Drawing on recent research of a multidisciplinary biocomplexity project, I explore in this article the Hawaiian archipelago as a model system for studying human ecodynamics. Natural patterns of biogeochemical and climate gradients constrained the development of intensive agroecosystems over 1,000 years. An early phase of exponential population growth was linked with agricultural intensification of terraced irrigation systems, primarily on the older islands. After C.E. 1400, expansion of population onto the leeward slopes of the young islands of Maui and Hawai'i was accompanied by intensification of dryland agricultural field systems. These changes were in turn linked to significant transformations of social and political formations, including restructuring of the system of land tenure and descent group organization, and the imposition of a system of surplus extraction organized around a ritual hierarchy of temples.     

采用酵母双杂交系统筛选GmDREB5的互作蛋白

以无自激活活性的GmDREB5蛋白73～226位氨基酸区段为诱饵,采用酵母双杂交系统筛选干旱处理5 h大豆cDNA文库.结果发现:一个互作蛋白含有保守的TPR(Tetratricopeptide repeat)结构域,与拟南芥的TPR蛋白仅有14%的相似性,说明其可能是一类新的大豆TPR蛋白,将其定名为GmTPR1;表达特性分析表明,GmTPR1基因受干旱、低温、高盐、ABA的诱导;证明GmTPR1不仅参与植物对非生物胁迫的响应,同时参与对GmDREB5蛋白水平的调控.     

Import Pathway of Nuclear-Encoded Cytochrome c Oxidase Subunit 2 Using Yeast as a Model

Abstract: Subunit 2 of cytochrome c oxidase (Cox2) is a mitochondrial-encoded protein in most organisms. In soybean Glycine max a second Cox2 gene was identified in the nucleus which is functional, whereas the mitochondrial-encoded cox2 gene is silent. For import and sorting of the nuclear-encoded soybean Cox2 protein ( Gm Cox2p) into mitochondria, the protein has acquired an N-terminal extension of 136 amino acid residues that is cleaved off in three steps during import. To study the function and processing of the Gm Cox2p leader peptide, we used yeast as a model system. Using different leader peptide-GFP constructs, we were able to show that the i₁ intermediate is generated in the mitochondrial matrix and the mature protein is generated in the inner membrane space. Mitochondrial processing peptidase (MPP) is involved in processing the first part of the leader peptide, processing of the last part is catalysed by the inner membrane peptidase (IMP). Oxa1p is necessary for insertion of the protein into the inner mitochondrial membrane. Gm Cox2p therefore utilises many of the same components as its mitochondrial-encoded predecessor, for sorting and maturation, following its import into the mitochondria.     

Coupling of Human DNA Excision Repair and the DNA Damage Checkpoint in a Defined in Vitro System

DNA repair and DNA damage checkpoints work in concert to help maintain genomic integrity. In vivo data suggest that these two global responses to DNA damage are coupled. It has been proposed that the canonical 30 nucleotide single-stranded DNA gap generated by nucleotide excision repair is the signal that activates the ATR-mediated DNA damage checkpoint response and that the signal is enhanced by gap enlargement by EXO1 (exonuclease 1) 5′ to 3′ exonuclease activity. Here we have used purified core nucleotide excision repair factors (RPA, XPA, XPC, TFIIH, XPG, and XPF-ERCC1), core DNA damage checkpoint proteins (ATR-ATRIP, TopBP1, RPA), and DNA damaged by a UV-mimetic agent to analyze the basic steps of DNA damage checkpoint response in a biochemically defined system. We find that checkpoint signaling as measured by phosphorylation of target proteins by the ATR kinase requires enlargement of the excision gap generated by the excision repair system by the 5′ to 3′ exonuclease activity of EXO1. We conclude that, in addition to damaged DNA, RPA, XPA, XPC, TFIIH, XPG, XPF-ERCC1, ATR-ATRIP, TopBP1, and EXO1 constitute the minimum essential set of factors for ATR-mediated DNA damage checkpoint response.     

利用毕赤酵母表达外源蛋白的研究

综述了毕赤酵母表达系统的优越性、表达受体菌和表达载体、酵母转化、分泌信号、翻译后加工和修饰等特点,以及广泛的医用、商业用途,在理论研究特别是蛋白质结构与功能：疗面的潜在应用价值。