Functional and structural characterization of a prokaryotic peptide transporter with features similar to mammalian PEPT1

The ydgR gene of Escherichia coli encodes a protein of the proton-dependent oligopeptide transporter (POT) family. We cloned YdgR and overexpressed the His-tagged fusion protein in E. coli BL21 cells. Bacterial growth inhibition in the presence of the toxic phosphonopeptide alafosfalin established YgdR functionality. Transport was abolished in the presence of the proton ionophore carbonyl cyanide p-chlorophenylhydrazone, suggesting a proton-coupled transport mechanism. YdgR transports selectively only di- and tripeptides and structurally related peptidomimetics (such as aminocephalosporins) with a substrate recognition pattern almost identical to the mammalian peptide transporter PEPT1. The YdgR protein was purified to homogeneity from E. coli membranes. Blue native-polyacrylamide gel electrophoresis and transmission electron microscopy of detergent-solubilized YdgR suggest that it exists in monomeric form. Transmission electron microscopy revealed a crown-like structure with a diameter of approximately 8 nm and a central density. These are the first structural data obtained from a proton-dependent peptide transporter, and the YgdR protein seems an excellent model for studies on substrate and inhibitor interactions as well as on the molecular architecture of cell membrane peptide transporters.     

DtpB (YhiP) and DtpA (TppB, YdgR) are prototypical proton-dependent peptide transporters of Escherichia coli

The genome of Escherichia coli contains four genes assigned to the peptide transporter (PTR) family. Of these, only tppB (ydgR) has been characterized, and named tripeptide permease, whereas protein functions encoded by the yhiP, ybgH and yjdL genes have remained unknown. Here we describe the overexpression of yhiP as a His-tagged fusion protein in E. coli and show saturable transport of glycyl-sarcosine (Gly-Sar) with an apparent affinity constant of 6.5 mm. Overexpression of the gene also increased the susceptibility of cells to the toxic dipeptide alafosfalin. Transport was strongly decreased in the presence of a protonophore but unaffected by sodium depletion, suggesting H(+)-dependence. This was confirmed by purification of YhiP and TppB by nickel affinity chromatography and reconstitution into liposomes. Both transporters showed Gly-Sar influx in the presence of an artificial proton gradient and generated transport currents on a chip-based sensor. Competition experiments established that YhiP transported dipeptides and tripeptides. Western blot analysis revealed an apparent mass of YhiP of 40 kDa. Taken together, these findings show that yhiP encodes a protein that mediates proton-dependent electrogenic transport of dipeptides and tripeptides with similarities to mammalian PEPT1. On the basis of our results, we propose to rename YhiP as DtpB (dipeptide and tripeptide permease B), by analogy with the nomenclature in other bacteria. We also propose to rename TppB as DtpA, to better describe its function as the first protein of the PTR family characterized in E. coli.     

Diploidy, evolution and sex

A new gene for a new purpose may be created by mutation of a pre-existing gene. But if that original gene is still required for its original purpose, and is to be retained side by side with the new, a spare copy is needed initially as raw material for the innovation. Thus in haploids the original gene must be duplicated before it is modified. But in diploids a spare copy of every gene is always available, and a mutant allele serving a new purpose can be easily established and maintained by heterosis in parallel with the old allele. Subsequent gene duplication will lead, via crossing-over, to insertion of the new gene in tandem with the old, as a permanent addition to the genome. Calculations show that diploids can thus enlarge their genomes with new genes for new purposes much more readily than haploids; in particular, they can more easily evolve the complex gene control systems characteristic of differentiated multicellular organisms. Sexual reproduction preserves diploidy, and so can be seen as the basis of these richer possibilities for evolutionary innovation.     

Cloning and characterization of the gene encoding the z66 antigen of Salmonella enterica serovar Typhi

Z66 antigen-positive strains of Salmonella enterica serovar Typhi change flagellin expression in only one direction from the z66 antigen to the d or j antigen, which is different from the phase variation of S. enterica serovar Typhimurium. In the present study, we identified a new flagellin gene in z66 antigen-positive strains of S. enterica serovar Typhi. The genomic structure of the region containing this new flagellin gene was similar to that of fljBA operon of biphasic S. enterica serovars. A fljA-like gene was present downstream of the new flagellin gene. A rho-independent terminator was located between the new flagellin gene and the fljA-like gene. Hin-like gene was not present upstream of the new flagellin gene. We generated a mutant strain of S. enterica serovar Typhi, which carries a deletion of the new flagellin gene. Western blotting revealed that the 51-kDa z66 antigen protein was absent from the population of proteins secreted by the mutant strain. Southern hybridization demonstrated that the z66 antigen-positive strains of S. enterica serovar Typhi carried the new flagellin gene and fliC on two different genomic EcoRI fragments. When z66 antigen-positive strains were incubated with anti-z66 antiserum, the flagellin expression by S. enterica serovar Typhi changed from z66 antigen to j antigen. The new flagellin gene and the fljA-like gene were absent in the strain with altered flagellin expression. These results suggested that the new flagellin gene is a fljB-like gene, which encodes the z66 antigen of S. enterica serovar Typhi, and that deletion of fljBA-like operon may explain why S. enterica serovar Typhi alters the flagellin expression in only one direction from the z66 antigen to the d or j antigen.     

Natural selection on gene order in the genome reorganization process after whole-genome duplication of yeast

A genome must locate its coding genes on the chromosomes in a meaningful manner with the help of natural selection, but the mechanism of gene order evolution is poorly understood. To explore the role of selection in shaping the current order of coding genes and their cis-regulatory elements, a comparative genomic approach was applied to the baker's yeast Saccharomyces cerevisiae and its close relatives. S. cerevisiae have experienced a whole-genome duplication followed by an extensive reorganization process of gene order, during which a number of new adjacent gene pairs appeared. We found that the proportion of new adjacent gene pairs in divergent orientation is significantly reduced, suggesting that such new divergent gene pairs may be disfavored most likely because their coregulation may be deleterious. It is also found that such new divergent gene pairs have particularly long intergenic regions. These observations suggest that selection specifically worked against deletions in intergenic regions of new divergent gene pairs, perhaps because they should be physically kept away so that they are not coregulated. It is indicated that gene regulation would be one of the major factors to determine the order of coding genes.     

cDNA微阵列技术在植物功能基因组学研究中的应用

cDNA微阵列 (cDNAMicroarrays)技术是近年发展起来的分子生物学研究新型工具 ,以分子杂交为基本原理 ,在检测植物基因表达水平、研究基因表达图谱、特异基因检测以及发现新基因和分离差异表达基因等方面有着独特的优势 ,已成为植物功能基因组学研究的重要手段。     

Phage genes involved in the formation generalized transducing particles in Salmonella--Phage P22

Summary Phage P22-mutants with increased or decreased ability to produce transducing particles (HT-¹ and NT-mutants) were submitted to mapping experiments. The gene responsible for HT-phenotype was found to be allelic to gene 3 of the P22 linkage map. For the NT-phenotype different genes were identified: gene 1 (or a new gene extremely close to it), gene 5, gene 8 and a new gene between genes 3 and 19.     

pUC19K质粒的构建及其在布鲁氏菌突变株构建中的应用

突变株的构建是细菌基因功能研究的前提。本研究构建了一个可用于布鲁氏菌突变株构建的自杀质粒。在pUC19质粒的多克隆位点插入卡那霉素抗性基因,在该基因两侧添加多个酶切位点,构建成为pUC19K。利用该质粒,我们构建了布鲁氏菌外膜蛋白Omp25基因的突变株。结果表明,利用该自杀质粒,通过一轮筛选即可得到目标基因被抗性基因替换的突变株。pUC19K质粒的构建及成功应用,为布鲁氏菌突变株的构建提供了一个快速有效的手段,也为布鲁氏菌的基因功能研究奠定了基础。     

功能基因组学技术在慢性疼痛研究中的应用

慢性疼痛是一个世界性难题,其治疗效果不佳,与其机制不明有很大关系。解决机制问题,探索有效的治疗方法已经成为研究的焦点。伴随着后基因时代的到来,以及分子生物学,生物信息学等多门生物相关学科的发展,RNA干扰技术,反义寡核苷酸技术,基因芯片等这些功能基因组学中常用的实验手段,通过在基因组或系统水平上全面分析基因的功能,为研究慢性疼痛发生机制,发现新的疼痛调节相关基因以及探索疼痛治疗的新途径开辟了更加广阔的空间。     

How is a species kept together?

Over the decades, there has been substantial empirical evidence showing that the unity of species cannot be maintained by gene flow. The biological species concept is inconclusive on this point. The suggestion is made that the unity of species is maintained rather by selection constantly spreading new alleles throughout the species, or bygene circulation. There is a lack in conceptual distinction between gene flow and gene circulation which lies at the heart of the problem. The concept of gene circulation also sheds some new light on the problem of typology and on such a broad concept as evolution. A new species definition is proposed.     

基因编辑技术

基因编辑是指通过核酸酶对靶基因进行定点改造,实现特定DNA的定点敲除、敲入以及突变等,最终下调或上调基因的表达,以使细胞获得新表型的一种新型技术。基因编辑技术已被广泛运用于基因结构与功能的研究和多种细胞的基因工程改造,为疾病模型的建立、动植物新品种的培育及基因治疗等的研究提供新的手段。基因编辑技术主要包括锌指核酸酶技术(ZFN)、转录激活子样效应因子技术(TALEN)和成簇的规律间隔的短回文重复序列/CRISPR相关蛋白 (CRISPR/Cas) 系统等。本文将对3种基因编辑技术的原理、运用及其最新进展进行综述,以期为相关技术及其运用的研究提供参考。     

Novel non-viral vectors for gene delivery: synthesis of a second-generation library of mono-functionalized poly-(guanidinium)amines and their introduction into cationic lipids

The development of new gene delivery technologies is a prerequisite towards gene therapy clinical trials. Because gene delivery mediated by viral vectors remains of limited scope due to immunological and propagation risks, the development of new non-viral gene delivery systems is of crucial importance. We have synthesized a secondary library of mono-functionalized poly-(guanidinium)amines generated from a library of mono-functionalized polyamines applying the concept of "libraries from libraries." The method allows a quick and easy access to mono-functionalized geometrically varied poly-(guanidinium)amines. The new building blocks were introduced into cationic lipids to obtain novel poly-(guanidinium)amine lipids, which are potential DNA vectors for gene delivery.     

Problems and paradigms: Induction mechanism of a single gene molecule: Stochastic or deterministic?

A new field of gene expression regulation research is emerging that has previously been overlooked. This new area is concerned with distinguishing the expression of a single gene from the averaged expression of many gene copies within the cell population. This paper reviews research focused on individual genes in inducible gene expression systems. The main experimental strategy is to measure the gene expression level of a single cell containing a single reporter gene molecule. In contrast to the commonly held belief, gene induction is found to be stochastic under certain conditions. The possible mechanisms and implications are discussed.     

Reshaping of global gene expression networks and sex-biased gene expression by integration of a young gene

New genes originate frequently across diverse taxa. Given that genetic networks are typically comprised of robust, co-evolved interactions, the emergence of new genes raises an intriguing question: how do new genes interact with pre-existing genes? Here, we show that a recently originated gene rapidly evolved new gene networks and impacted sex-biased gene expression in Drosophila. This 4–6 million-year-old factor, named Zeus for its role in male fecundity, originated through retroposition of a highly conserved housekeeping gene, Caf40. Zeus acquired male reproductive organ expression patterns and phenotypes. Comparative expression profiling of mutants and closely related species revealed that Zeus has recruited a new set of downstream genes, and shaped the evolution of gene expression in germline. Comparative ChIP-chip revealed that the genomic binding profile of Zeus diverged rapidly from Caf40. These data demonstrate, for the first time, how a new gene quickly evolved novel networks governing essential biological processes at the genomic level.     

基因组重排技术在开发新代谢产物中的应用

基因组重排是一种基于原生质体融合,并对原生质进行递推式融合的新型技术。随着基因组重排技术的不断发展和成熟,通过基因组重排获得新代谢产物的例子不断出现,表明该项技术作为新代谢产物开发的途径具有一定的应用前景。在此列举了基因组重排在开发新代谢产物方面的成果,包括基因组重排激活沉默基因产生新代谢产物;基因组重排引入单酶基因产生新抗生素;基因组重排互换基因模块产生杂合抗生素和基因组重排替换前体基因产生新抗生素的例子,并展望了其发展的趋势。     

一株链霉菌菌株NCPC-1020中棘白霉素B脱酰基酶基因的克隆与功能分析

【目的】从一株土壤放线菌来源的野生型链霉菌菌株NCPC-1020中克隆一个具有棘白霉素B脱酰基酶活性的新基因。【方法】采用Degenerate和TAIL PCR两种方法,从链霉菌菌株NCPC-1020基因组中快速克隆获得了该基因序列,然后将基因在变铅青链霉菌TK24中进行异源表达,并进行全细胞催化底物脱酰基反应,采用LC-MS检测反应产物。【结果】LC-MS检测证实,棘白霉素B结构中脂肪链被酶促水解,从而证实该基因具有脱酰基酶活性。【结论】采用Degenerate以及TAIL PCR的方法能够快速获得未知功能的新基因。此基因的克隆,奠定了进行半合成棘白霉素类药物的研发基础。     

A human gene encoding a protein homologous to ribosomal protein L39 is normally expressed in the testis and derepressed in multiple cancer cells

We identified and characterized a gene encoding a protein that was 92% identical to human ribosomal protein L39. This gene was located on the long arm of chromosome 3, and was composed of three exons and two long introns. Analysis of mRNA expression in 16 types of normal human tissues showed that this gene was expressed specifically in the testis, in sharp contrast to the ubiquitous expression of the ribosomal protein L39 gene. Surprisingly, the new gene was expressed in 19 out of 24 human cancer samples of various tissue origins. When the new gene was expressed in the cell, a translated product was observed by immunofluorescence microscopy in the nucleus, especially strongly in the nucleolus, and in the cytoplasm. Association of this protein with the large subunit of cytoplasmic ribosomes was detected by polyacrylamide-agarose composite gel electrophoresis followed by immunodetection. These immunochemical data suggest a relationship between the new gene and the ribosome.     

一个新葡萄糖淀粉酶基因的克隆与表达

根据已报道的米根霉葡萄糖淀粉酶基因序列,通过PCR方法,从天然少根根霉的总DNA中克隆到含有四个内含子的葡萄糖淀粉酶基因。通过设计引物并采取重叠PCR方法删除内含子,获得了新的少根根霉葡萄糖淀粉酶(Rhizopus arrhizu glucoamylase,RaGA)cDNA序列(Accession number:DQ903853)。该基因在毕赤酵母中成功表达,表达产物具有较高的葡萄糖淀粉酶活性。     

水稻白叶枯病新抗源Y238的鉴定及其近等基因系培育

从269份普通野生稻中鉴定出一个高抗白叶枯病的新抗源,编号为Y238.通过多茵系鉴定、抗谱分析及与目前国际上已知基因比较,证明该新抗源含有一个新基因,暂命名为WBB2.对JG30/Y238杂交后代成株期接种鉴定、遗传分析表明,WBB2为完全显性基因.通过杂交和回交,已将WBB2导入栽培稻中构建近等基因系.