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1.
以念珠藻属(Nostoc)及其近缘类群hetR基因的51条序列为研究对象,对hetR基因的编码蛋白进行生物信息学分析和系统发育分析,并使用分支模型、位点模型和分支-位点模型进行该基因位点的适应性进化研究。系统发育分析结果显示,51条hetR基因蛋白序列可分为4个大分支。适应性进化分析结果表明,在3种进化模型中,大多数分支及藻株都没有检测到统计学上具有显著性的正选择位点,说明检测的位点大多处于负选择压力下。但在普通念珠藻(Nostoc commune,CHAB2802)中检测到正选择位点(126T),提示念珠藻属植物hetR基因发生了适应性改变。  相似文献   

2.
蕨类植物rbcL基因正选择和负选择位点的鉴定   总被引:1,自引:0,他引:1  
基于分支模型、位点模型及分支-位点模型对蕨类的rbcL基因所受到的选择压力进行了分析.结果显示:分支模型下检测到大部分分支处于负选择,仅4个分支处于正选择压力下,并且仅2分支具有统计上的显著性;在位点模型下,通过比较模型M1a/M2a和M7/M8,在氨基酸水平上模型M2a和模型M8均鉴定出98L位点被正选择;在模型M8下,鉴定负向选择位点共228个,占总序列的83.82%,从而揭示出负选择对rbcL基因的进化起着非常重要的作用;在分支位点-模型c下鉴定出262A被正选择.98L、262A位点分别位于rbcL羧基末端α/β桶结构域的第3和第8个α螺旋上.蕨类通过该结构域的适应性进化,适应白垩纪被子植物兴起而引发的陆地生态系统改变,研究结果为以后实验分析提供了首选位点.  相似文献   

3.
为探讨淡水红藻的叶绿体基因及其适应性进化特征,选取弯枝藻属(Compsopogon)及相近外类群的rbc L基因共17条,利用PAML 4.9软件,对弯枝藻属rbc L基因编码蛋白进行生物信息学分析,并分别采用分支模型、位点模型以及分支-位点模型对基因的选择位点进行检测。结果表明,弯枝藻属rbc L基因编码蛋白的二级结构主要由α螺旋和β折叠构成,结构稳定。采用最大似然法构建的系统发育树表明,内类群为单一物种,分为3个小分支,具有一定地理分布规律。在3种进化模型中均未检测到统计上显著的正选择位点,表明绝大多数位点处于负选择压力下。因此,弯枝藻属rbc L基因未发生适应性进化。  相似文献   

4.
大黄属(Rheum L.)是蓼科(Polygonaceae)中一个高度分化的大属,广泛分布在亚洲和欧洲的高山和沙漠地区,全世界约60种,其中在青藏高原及其邻近地区发现了约40种。该属种的高度分化曾被推测是第三纪末青藏高原的快速隆升以及第四纪气候的反复变化所引发的适应性辐射导致。为进一步了解大黄属植物辐射式物种分化的分子适应机制,该研究选取34个形态上多样化的大黄属物种,利用系统发育分析软件,在时间框架下采用位点模型和分支模型对大黄属的叶绿体ndhF基因进行了适应性进化分析。结果表明:大黄属植物的分子进化系统树呈现短而平行的辐射式分支式样,显示出典型的物种快速辐射多样化特征;用位点模型检验ndhF基因是否存在经受正向选择(ω>1)时,在氨基酸水平上共鉴定出3个NDHF亚基的正选择位点(188H,465H,551L),对NDHF亚基的二级结构进行分析后发现编码的188H氨基酸位于α螺旋上。大黄属植物可能通过这些结构域的适应性进化,适应青藏高原的快速隆升以及第四纪气候的反复变化而引发的陆地生态系统改变。该研究结果可为今后对该属植物的实验分析提供首选位点。  相似文献   

5.
凤尾蕨科植物rbcL基因的适应性进化分析   总被引:2,自引:0,他引:2  
为深入理解蕨类植物辐射式物种分化的分子适应机制,在时间框架下,采用位点模型和分支-位点模型对凤尾蕨科植物rbcL基因的进化式样进行了分析.通过比较模型M1a/M2a和M7/M8,在氨基酸水平上共鉴定出6个正选择位点:1491、251M、255V、282F、359S和375F,其中位点282F对维持Rubisco功能有重要作用.分别检验凤尾蕨科的附生分支和水蕨类分支发现,前者不具适应性进化位点,而后者有两个位点(230A和247C)经历正选择.相对于荫蔽的光条件,水生生境可能对RbcL亚基的选择作用更强.另外,基于UCLD分子钟模型估算出的风尾蕨科各分支分化时间表明,该科物种丰富度的辐射式增长发生在新生代渐新世,推测古、始新世最热事件可能对物种分化的形成也产生一定作用.这对认识薄囊蕨类如何应对被子植物兴起导致的陆地生态系统改变具重要意义.  相似文献   

6.
3种水稻土中7株固氮蓝细菌的分离与特征   总被引:1,自引:0,他引:1       下载免费PDF全文
【背景】蓝细菌是水生和陆地生态系统中生物固氮的主要贡献者。【目的】增加对稻田土壤固氮蓝细菌的了解,获得用于进一步研究的可培养固氮蓝细菌菌株。【方法】选择3种具有不同固氮能力的水稻土,采用BG11-N培养基分离培养固氮蓝细菌菌株,对新分离菌株进行形态特征观察,通过基因组DNA的nifH基因扩增明确其固氮潜力,进一步采用乙炔还原法和~(15)N_2示踪法定量测定其固氮能力,通过基因组DNA的16SrRNA基因序列比对进行鉴定。【结果】在光照培养条件下,采用BG11-N培养基共分离纯化得到自养菌株7株,细胞呈圆形或椭圆形、单列、无分枝、丝状和念珠状,在固体培养基上形成团垫状菌落。新分离菌株在BG11-N培养基中生长状况良好,以基因组DNA为模板可扩增出nifH基因,乙炔还原法和~(15)N_2示踪法测定结果显示具有较高固氮能力,同时具有铁载体生成能力。结合16S rRNA基因序列比对和形态特征,7株菌被初步鉴定隶属于念珠藻科(Nostocaceae)。【结论】从水稻土中分离到在稻田生物固氮中发挥重要作用的蓝细菌(念珠藻科)菌株,可培养固氮蓝细菌菌株固氮能力较高,兼具铁载体生成能力,可作为进一步深入研究的微生物资源,具有潜在的研究应用价值。  相似文献   

7.
弗兰克氏菌(Frankia)因其独特高效的固氮效率而备受关注,然而目前的研究还局限于陆地生境。基于nifH基因采用高通量测序对高隆湾红树林及其近岸海域沉积物的Frankia多样性进行分析,共获得261条属于Frankia的nifH序列,共11个OTUs,序列主要分布在红树林区样品,其中以角果木和红海榄为优势树种的红树林样品中序列较多,在潮间带样品中也有少量分布,海草区样品未检测到,序列在不同生境中的分布存在较大差异。OTU818在10个站位都有分布,说明OTU818代表的Frankia类群分布比较广泛,且为红树林沉积物的优势类群。系统进化分析表明Frankia与NCBI数据库中的Frankia基因序列在系统发育树上形成不同分支。通过Network分析Frankia与其他细菌类群的共发生关系,发现Frankia与来自Verrucomicrobia、Proteobacteria、Firmicutes、Cyanobacteria的多种固氮细菌类群存在紧密联系,表明Frankia在稳定红树林固氮细菌群落结构中起着重要作用。利用典范对应分析(canonical correspondence an...  相似文献   

8.
【目的】采用多位点序列分析方法,研究印度洋3 000 m以下深海沉积物中分离得到的16S rRNA基因比对高度相似的链霉菌菌株的种间系统发育关系,同时探讨各管家基因及多基因聚类分析后的种间区分能力。【方法】以分离自印度洋深海沉积物的7株Streptomyces albidoflavus,11株Streptomyces cavourensis,16株Streptomyces pratensis为研究对象,以16S rRNA、atpD、recA和rpoB基因片段为标记,通过PCR扩增、测序,获得序列。同时从NCBI上下载5株S.pratensis上述4个基因的序列,将所有序列在MLST网站进行比对,并构建系统进化树进行比较。【结果】S.pratensis各菌株种内比较发现,16S rRNA基因构建的系统进化树中相同基因型的菌株没有聚在一起,系统进化树不稳定,区分度不高。其余3个构建的系统进化树稳定,菌株的聚类关系与MLST数据库得到的基因型一致。同时,多基因聚类分析后将菌株分为6个类群。在3个种的种间多位点序列比较中,除区分度明显增加、进化树更加稳定以外,还发现rec A基因进化上比较特殊的菌株。【结论】多位点序列分析将实验菌株分为很多不同的类型,成功地将所分离的链霉菌进行了更细的分类,同时也找到部分菌株在个别基因上差异较大。此方法可以用于相近种的快速鉴定。  相似文献   

9.
采用非变性聚丙烯酰胺凝胶电泳,对90份小麦品种的淀粉分支酶同工酶(SBE)进行检测,以分析不同基因型对支链淀粉含量的遗传效应.结果表明:(1)SBEⅠ型显现出较为丰富的变异,具有A、B、Dⅰ和Dⅱ4个等位基因位点;SBEⅡ型仅具有SBEⅡa单一等位基因位点.根据SBEⅠ型4个基因位点在不同品种中的分布,可将90个品种分为7种基因型.不同基因型对支链淀粉含量的遗传效应分析表明,含有A位点的基因型(ADⅰDⅱ和ADⅰB)所对应的支链淀粉含量较高,且与由1个基因位点组成的基因型(Dⅰ)和2个基因位点组成的基因型(DⅰB和DⅰDⅱ)的支链淀粉含量差异显著.  相似文献   

10.
为明确葛仙米(Nostoc sphaeroides)中血红素氧合酶(Heme oxygenase, HO)基因编码蛋白的分子进化地位和高级结构, 克隆该基因并进行原核细胞表达, 氨基酸序列比对与分子进化分析和Swiss-model高级结构模拟。结果显示: 葛仙米血红素氧合酶基因Ns-HO1密码区全长为678 bp, 预编码一含225个氨基酸的蛋白质; Ns-HO1与同源蛋白氨基酸相似性达90.3%, 存在少部分位点替换突变, 但底物血红素的预结合位点(如Arg10和Tyr125)及金属离子结合位点(His17)等关键位点的氨基酸保持稳定。 构建表达载体, 葛仙米Ns-HO1在大肠杆菌中成功诱导表达, SDS-PAGE检测目的蛋白大小近26.0 kD; 分子进化树分析显示Ns-HO1与普通念珠藻、发状念珠藻中同源蛋白聚类于同一分支, 并与点状念珠藻中同源蛋白具有共同祖先。Ns-HO1蛋白多肽链形成8个主要α-螺旋,其中N和C末端的两个α-螺旋与第四螺旋共同为Ns-HO1高级结构提供底面支撑, 其他螺旋围绕该底面进一步延展并充填其中, 形成Ns-HO1分子的类夹心式结构。在高级结构中, 含血红素预结合位点氨基酸的几个螺旋(第一、 五和七螺旋)位于Ns-HO1分子外围, 这些分支螺旋为形成Ns-HO1夹心空间以利于底物血红素锚定和产物及时释放提供了条件。总之, 研究为深入了解与运用葛仙米血红素氧合酶基因的生物学功能和资源提供了基础。  相似文献   

11.
Hierarchical clustering and similarity coefficients of pairwise alignments of the published nucleotide sequences of 27nifH genes suggest thatnif genes are as ancient as the archaebacteria and clostridia. The positions ofnifHl ofMethanococcus thermolithotrophicus, nifH3 ofClostridium pasteurianum, nifH3 ofAzotobacter vinelandii andnifH ofFrankia suggest that a variety of lateral transfers may have occurred during evolution ofnifH gene. The genes for type 3 nitrogenase ofA. vinelandii may have diverged early from methanogens and clostridia. A high similarity coefficient with the derived amino acid sequence of type 3 nitrogenase suggests the presence of a functionally similar enzyme inC. pasteurianum. The type 2 nitrogenase genenifH2 of azotobacters seems to have originated recently from the genenifHl for conventional type I nitrogenase. RhizobialnifH genes comprise two closely related but discrete clusters that are in consonance with the plasmid or chromosomal location ofnif genes. The chromosomal and plasmid locatednifH of rhizobia seem to have evolved independently but contemporaneously.  相似文献   

12.
The sizes of endonuclease digestion fragments of DNA from cyanobacteria in symbiotic association with Azolla caroliniana or Anthoceros punctatus, or in free-living culture, were compared by Southern hybridization using cloned nitrogenase (nif) genes from Anabaena sp. PCC 7120 as probes. The restriction fragment pattern produced by cyanobacteria isolated from A. caroliniana by culture through symbiotic association with Anthoceros differed from that of the major symbiotic cyanobacterium freshly separated from A. caroliniana. The results indicate that minor cyanobacterial symbionts occur in association with Azolla and that the dominant symbiont was not cultured in the free-living state. Both the absence of hybridization to an xisA gene probe and the mapping of restriction fragments indicated a contiguous nifHDK organization in all cells of the symbiont in association with Azolla. On the other hand, in the cultured isolate from Azolla and in Nostoc sp. 7801, the nifD and nifK genes are nominally separated by an interval of unknown length, compatible with the interruption of the nifHDK operon by a DNA element as observed in Anabaena sp. PCC 7120. In the above cultured strains, restriction fragments consistent with a contiguous nifHDK operon were also present at varying hybridization intensities, especially in Nostoc sp. 7801 grown in association with Anthoceros, presumably due to gene rearrangement in a fraction of the cells.Non-standard abbreviations bp base pairs - kb kilobase pairs - kd kilodaltons  相似文献   

13.
A small plasmid containing the entire nif gene cluster of Enterobacter agglomerans 333 as an excisable cassette has been constructed, using pACYC177 as a vector. Two cosmid clones taken from a gene library of E. agglomerans plasmid pEA3 were used as a source of nif genes. A SmaI fragment of peaMS2-2, containing the H,D,K,Y,E,N,X,U,S,V,W,Z,M,L,A and B genes and an ApaI fragment of peaMS2-16 containing nifA,B,Q,F and J were selected to construct pMH2. The resulting plasmid of 33 kb carries the complete nif gene cluster as a nif cassette on a single XbaI fragment. The nif construct pMH2 in Escherichia coli strains has significant nitrogenase activity compared to wild-type E. agglomerans 333. The nif gene cluster construct was found to be very stable.  相似文献   

14.
[目的]来自Paenibacillus polymyxa WLY78的固氮基因簇(nifBHDKEfNXhesAnifV)可以转化入Escherichia coli中表达并使重组大肠杆菌合成有固氮活性的固氮酶。本文拟通过对重组大肠杆菌E.coli 78-7的转录组分析以提高其固氮能力。[方法]对固氮条件(无氧无NH4+)和非固氮条件(空气和100 mmol/L NH4+)培养的重组大肠杆菌E.coli 78-7进行转录组分析。[结果]nif基因在两种培养条件下显著表达,说明在重组大肠杆菌中可规避原菌中氧气和NH4+nif基因的负调控。对于固氮过程必需的非nif基因,如参与钼、硫、铁元素转运的modcysfeoAB,这些基因在两种培养条件下表达水平有差异。而参与铁硫簇合成的sufisc基因簇在两条件下表达水平差异巨大。此外,参与氮代谢的基因在固氮条件下显著上调。[结论]重组大肠杆菌中与固氮相关的非nif基因在该菌的固氮过程中具有较大影响,本文对在异源宿主中调高固氮酶活性研究具有重要意义。  相似文献   

15.
Strains of the obligately aerobic nitrogen fixing organismAzotobacter chroococcum were constructed which contained defined chromosomal deletions in which the nitrogenase structural genenifHDK cluster (nifH for the polypeptide of the Fe-protein component of nitrogenase andnifD andnifK for the alpha and beta subunits respectively of the MoFe-protein component of the enzyme) was replaced by a kanamycin resistance gene. N2 fixation was nevertheless observed in deletion strains though only in a molybdenum-deficient medium or in spontaneously arising tungstate-resistant derivatives. In comparison with the parent strain growing in molybdenum-sufficient medium, diazotrophic growth was slow and the nitrogenase activity in vivo was characterised by disproportionately low rates of C2H2-reduction compared to H2-evolution and relative insensitivity of H2-evolution to inhibition by C2H2. The findings show reiteration of functional structural genes for nitrogenase inA. chroococcum consistent with our previous observation of twonifH genes in this organism and detection in this work of a secondnifK-like sequence in the genomes of both parent and deletion strains whenA. chroococcum nifK DNA was used as a probe.  相似文献   

16.
It was known that nitrogenase genes and proteins are well conserved even though they are present in a large variety of phylogenetically diverse nitrogen fixing bacteria. This has lead to the speculation, among others, that nitrogen fixation (nif) genes were spread by lateral gene transfer relatively late in evolution. Here we report an attempt to test this hypothesis.We had previously established the complete nucleotide sequences of the three nitrogenase genes from Bradyrhizobium japonicum, and have now analyzed their homologies (or the amino acid sequence homologies of their gene products) with corresponding genes (and proteins) from other nitrogen fixing bacteria. There was a considerable sequence conservation which certainly reflects the strict structural requirements of the nitrogenase iron-sulfur proteins for catalytic functioning. Despite this, the sequences were divergent enough to classify them into an evolutionary scheme that was conceptually not different from the phylogenetic positions, based on 16S rRNA homology, of the species or genera harboring these genes. Only the relation of nif genes of slow-growing rhizobia (to which B. japonicum belongs) and fast-growing rhizobia was unexpectedly distant. We have, therefore, performed oligonucleotide cataloguing of their 16S rRNA, and found that there was indeed only a similarity of S AB=0.53 between fast- and slowgrowing rhizobia.In conclusion, the results suggest that nif genes may have evolved to a large degree in a similar fashion as the bacteria which carry them. This interpretation would speak against the idea of a recent lateral distribution of nif genes among microorganisms.  相似文献   

17.
Non-heterocystous, non-nitrogenfixing (het - nif-), heterocystous, non-nitrogenfixing (het + nif-) and multiple heterocystous, nitrogen-fixing (M-het + nif+) mutants of heterocystous, nitrogen-fixing (het + nif+) wild-type Nostoc muscorum and Nostoc linckia were isolated and characterized with respect to (a) nitrogenfixing activity, (b) reversion frequency, (c) ammonium repressibility of heterocyst formation, (d) heterocyst spacing pattern, and (e) action of L-methionine-DL-sulphoximine (MSO), an inhibitor of glutamine synthetase (GS), on heterocyst regulation. The mutant and revertant results suggest: (i) either involvement of a common genetic determinant in the formation of heterocyst and nitrogenase or the organization of het genes and nif genes in a single operon prone to complete inactivation by a single polar mutation, (ii) non-participation of active nitrogenase in regulation of heterocyst spacing; (iii) involvement of genetic factor(s) in the control of heterocyst spacing pattern in N. linckia, and (iv) apparently different nature of the mechanism of heterocyst inhibition by proheterocyst from that of heterocyst inhibition by NO 3 - or NH 4 + . L-Methionine-DL-sulphoximine inhibits growth and causes heterocyst formation in chains in N. linckia growing in nitrogen-free, NO 3 - , NO 2 - or NH 4 + medium, thus indicating a close physiological linkage between heterocyst and inorganic nitrogen metabolism regulation.  相似文献   

18.
Summary Labeled probes carrying the Anabaena PCC 7120 nitrogenase (nifK and nifD) and nitrogenase reductase (nifH) genes were hybridized to Southern blots of DNA from diverse N2-fixing cyanobacteria in order to test a previous observation of different nif gene organization in nonheterocystous and heterocystous strains. The nif probes showed no significant hybridization to DNA from a unicellular cyanobacterium incapable of N2 fixation. All nonheterocystous cyanobacteria examined (unicellular and filamentous) had a contiguous nifKDH gene cluster whereas all of the heterocystous strains showed separation of nifK from contiguous nifDH genes. These findings suggest that nonheterocystous and heterocystous cyanobacteria have characteristic and fundamentally different nif gene arrangements. The noncontiguous nif gene pattern, as shown with two Het- mutants, is independent of phenotypic expression of heterocyst differentiation and aerobic N2-fixation. Thus nif arrangement could be a useful taxonomic marker to distinguish between phenotypically Het- heterocystous cyanobacteria and phylogenetically unrelated nonheterocystous strains.  相似文献   

19.
An EcoRI fragment of Rhizobium meliloti M2011 which shows homology to Klebsiella pneumoniae DNA carrying nifH and nifD was cloned in both orientations into the Cm gene of plasmid pACYC184 and expressed in Escherichia coli minicells. Fragment specific polypeptides of Mr 12 500, 21 000, 30 000, and 31 000 could be identified. By transposon mutagenesis it was shown that two of them (Mr 12 500 and 21 000) are fusion products with parts of the chloramphenicol acetyltransferase. The other two polypeptides are specified by one coding region which could be mapped by transposon mutagenesis. There are several reasons (homology to Klebsiella nifH, sequence data and molecular weight of the gene products) to assume that this coding region represents the R. meliloti nifH gene (gene for the subunit of the R. meliloti nitrogenase reductase, RmII).  相似文献   

20.
Summary The 17 kb region between the Bradyrhizobium japonicum nitrogenase genes (nifDK and nifH) was investigated for the presence of further nif or fix genes by site-directed insertion or deletion/replacement mutagenesis and interspecies hybridization. Mutant strains were tested for their ability to reduce acetylene in free-living, microaerobic culture (Nif phenotype) and in soybean root nodules (Fix phenotype). The presence of a gene, previously identified by hybridization with the Klebsiella pneumoniae nifB gene, was proved by isolation of a nifB insertion mutant which was completely Nif- and Fix-. Three other regions were found to be homologous to the K. pneumoniae genes nifE, nifN, and nifS, NifE and nifN insertion mutants were completely Nif-/Fix- whereas nifS mutants were leaky with 30% residual Fix activity. Taken together, the data show that the B. japonicum genome harbours a cluster of closely adjacent genes which are directly concerned with nitrogenase function.  相似文献   

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