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1.
基于转录组分析铜绿假单胞菌DN1降解荧蒽特性   总被引:1,自引:0,他引:1  
[背景]铜绿假单胞菌DN1是一株从石油污染土壤中分离筛选到的具有广谱降解功能的菌株。[目的]深入了解荧蒽胁迫条件下铜绿假单胞菌DN1降解污染物过程中重要的降解相关基因信息。[方法]通过高通量测序技术对铜绿假单胞菌DN1进行转录组测序,对其所有的转录本进行KEGG (kyoto encyclopedia of genes and genomes)分类和Pathway注释、GO (gene ontology)分类和富集分析。[结果]转录组测序显示:与对照组相比,荧蒽诱导组检测到6 189个基因,其中1 919个基因上调表达,1 603个基因下调表达。KEGG注释分析显示差异上调表达基因匹配到了112个KEGG代谢途径,注释到"代谢途径"的1 408个基因(约占总差异基因的73.4%)中有317个基因参与了碳氢化合物代谢及含有苯环结构的异源生物质的生物降解,占"代谢途径"的16.53%,暗示了菌株DN1降解荧蒽可能与这些途径有密切关系。另外,主要代谢途径中的差异表达基因主要集中在ABC转运系统、氨基酸生物合成、双组分系统及碳代谢,这些途径大多数参与了底物的识别转运、信号转导及基因表达调控。[结论]进一步拓展了铜绿假单胞菌DN1在荧蒽胁迫条件下的代谢途径和逆境反应,也为微生物修复环境污染物研究夯实了理论基础。  相似文献   

2.
【目的】食烷菌是海洋烃类降解优势菌,其烷烃代谢调控机制有待深入研究。本研究拟从食烷菌转录和翻译水平上认识烷烃降解的调控过程。【方法】分别以乙酸和正十六烷(C16)为唯一碳源与能源,获取柴油食烷菌(Alcanivorax dieselolei) B5菌株的转录组和翻译组数据,并整合数据计算得到该菌在2种碳源培养条件下基因的翻译效率。采用基因本体论(gene ontology, GO)和京都基因和基因组百科全书(Kyoto encyclopedia of genes and genomes, KEGG)对差异翻译和翻译效率基因进行功能和代谢通路注释。【结果】当以C16为唯一碳源与能源时,B5菌株烷烃代谢途径的关键基因在转录与翻译水平均大量提升,包括烷烃单加氧酶、细胞色素P450氧化酶、醇脱氢酶和醛脱氢酶等。KEGG富集结果表明,翻译水平显著上调基因参与了肽聚糖生物合成、脂肪酸降解、氯代烷烃降解、氧化磷酸化和生物膜形成等通路;翻译效率差异基因主要富集在铁载体非核糖体肽的生物合成、氧化磷酸化和不饱和脂肪酸的生物合成等途径。通过转录组和翻译组学的联合分析显示,为了适应烷烃氧化,B5有效地协调了转...  相似文献   

3.
摘要:【目的】研究不同碳源,特别是联苯条件下红球菌的细胞转录应答,以挖掘与多氯联苯(PCBs)转运、代谢及其调控相关的基因,为进一步全面理解PCB微生物降解的分子机制奠定基础。【方法】以一株多氯联苯降解菌红球菌(Rhodococcus sp.R04)为材料,分别提取不同碳源(乙醇、葡萄糖和联苯)培养条件下菌体的总RNA,反转录合成cDNA。采用高通量测序法分别对这三种样品进行转录组测序,分析测序数据得出全基因组表达模式,并对不同条件下的基因表达进行差示分析,进而对联苯代谢网络和红球菌中其他基因的转录调节和代谢应答反应做出相关性分析。Q-RT-PCR分析不同碳源培养条件下的基因表达情况。【结果】测序结果表明,与葡萄糖和乙醇相比,联苯培养条件下明显上调(log2 Ratio 1)基因个数分别为375和332个。与葡萄糖相比,联苯培养条件下,相关基因上调表达量与Q-RT-PCR实验结果基本一致。功能分类获得细胞组分、分子功能和生物学过程三大类别160多个细小分支的差示表达基因,部分基因参与联苯代谢转录调控、联苯转运、抗氧化应激反应以及信号传导通路系统等多种生理过程。参与联苯上游代谢途径的众多同工酶基因中,只有bphC2和bphD1在联苯中大量上调表达,其余同工酶在联苯中基本量不变或下调表达。转录组注释及差示分析推测,红球菌R04中苯甲酸的代谢主要是通过儿茶酚邻位途径、间位途径以及原儿茶酸途径三条代谢途径完成。【结论】与葡萄糖和乙醇相比,红球菌R04在联苯培养条件下基因表达差异明显,这为我们进一步解析多氯联苯代谢特征和代谢调控提供理论依据。  相似文献   

4.
【背景】广叶绣球菌(Sparassis latifolia)是一种名贵的食用菌,其木质纤维素降解的分子机制尚不明确。【目的】了解广叶绣球菌在不同碳源条件下木质纤维素降解相关基因表达动态。【方法】通过转录组测序技术对分别以葡萄糖、纤维素+木质素、纤维素及松木屑为碳源的广叶绣球菌基因表达谱进行分析。以葡萄糖为碳源的样本为对照,分别对不同碳源下广叶绣球菌显著差异表达的基因进行功能分析。【结果】Geneontology(Go)富集分析表明,以葡萄糖为碳源的样本为对照,差异表达基因主要富集在碳水化合物利用的过程,如多糖催化过程、碳水化合物催化过程、碳水化合物代谢过程及多糖代谢过程等。碳水化合物活性酶(Carbohydrate-activeenzymes,CAZymes)功能注释表明,碳源种类主要影响了半纤维素和纤维素降解相关糖苷水解酶家族基因的表达,其中涉及半纤维素降解的相关酶基因上调幅度最大。同时,在纤维素+木质素、松木屑为碳源的处理组中一些转录因子基因上调表达显著。【结论】不同碳源显著影响了广叶绣球菌基因表达谱,这种对碳源的适应也可能反映了广叶绣球菌攻击植物细胞壁的机制,研究结果为深入了解广叶绣球菌木质纤维素降解的分子机理和相关功能基因提供了一些参考。  相似文献   

5.
为了研究烟草脉斑驳病毒(TVMV)侵染本氏烟的抗病分子机制,本文建立了TVMV转录组数据库,挖掘抗病相关基因以及代谢和信号通路,采用Illumina Novaseq 6000高通量测序平台对侵染TVMV的本氏烟进行转录组测序,并进行生物信息学分析;利用R package:edge R等软件分析了有关抗病的差异表达基因,对差异表达基因进行基因本体论(GO)及京都基因和基因组百科全书(KEGG)基于途径的通路富集分析。基于TVMV侵染本氏烟转录组的测序结果中共获得4 593个差异表达基因,其中3 564个基因上调表达,1 029个基因下调表达。共筛选出10个抗病相关的差异表达显著基因,6个上调,4个下调。GO数据库中注释到生物学过程、细胞组分及分子功能等三大类共50个功能组。其中,在第三大类分子功能中,蛋白质结合功能以及ATP结合功能所涉及的差异表达基因最显著,分别为501个和453个差异基因。KEGG共富集20条通路,注释到核糖体途径的差异基因富集程度最高,基因最显著,差异表达基因数为307个。蛋白质结合、ATP结合、核糖体、真核生物核糖体的生物反应、DNA复制(DNA replicat...  相似文献   

6.
为探讨巴氏蘑菇子实体不同发育阶段基因的表达情况,本研究对巴氏蘑菇子实体不同发育时期(原基、采收期和开伞期)进行转录组测序,以本实验室已获得的巴氏蘑菇JA菌株的不育单孢菌株JA-15036基因组为参考基因组研究原基与采收期及开伞期样本间差异表达基因,并对差异表达基因进行了GO功能和Pathway富集分析。GO功能分析结果显示,差异表达基因主要富集在跨膜转运、碳水化合物代谢途径和膜组分,它们协同调控为子实体生长发育提供稳定的内环境。KEGG富集分析结果表明,原基期上调的差异表达基因主要富集在核糖体蛋白和DNA复制,表明原基期细胞代谢旺盛,其中核糖体蛋白基因上调为后期蛋白质合成提供重要场所;采收期和开伞期子实体时期差异表达基因主要富集在碳水化合物代谢、脂肪酸降解和氨基酸代谢等途径,为巴氏蘑菇子实体的生长发育与成熟提供营养与能量。  相似文献   

7.
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8.
新分离Microbacteriumsp.XT11菌能够合成黄原胶降解酶,将植物病原菌野油菜黄单孢菌分泌的毒素因子黄原胶分解,生成具有激发子和抗微生物活性的黄原胶寡糖。实验确认,黄原胶和酵母浸粉分别是XT11菌生产黄原胶降解酶的最适碳源和氮源,获得最高酶活力的最低碳源和氮源浓度均为0.3%。XT11菌生产黄原胶降解酶的最适条件为:培养温度28℃,培养基起始pH7.0,转速150r/min。  相似文献   

9.
新分离Microbacterium sp.XT11菌能够合成黄原胶降解酶,将植物病原菌野油菜黄单孢菌分泌的毒素因子黄原胶分解,生成具有激发子和抗微生物活性的黄原胶寡糖。实验确认,黄原胶和酵母浸粉分别是XT11菌生产黄原胶降解酶的最适碳源和氮源,获得最高酶活力的最低碳源和氮源浓度均为0.3%。XT11菌生产黄原胶降解酶的最适条件为:培养温度28℃,培养基起始pH7.0,转速150r/min。  相似文献   

10.
漆酶是香菇生长发育过程中一种重要的木质素降解酶,其活性高低对于香菇木质素降解能力和香菇品质形成具有重要作用。为探讨香菇不同漆酶活性的单核菌丝体基因表达变化,对漆酶活性存在差异的单核菌丝体进行转录组测序分析,共获得15 522个注释基因。GO(gene ontology)分析表明差异基因在氧化还原酶活性节点大量富集,包括参与木质素降解的酶类及55个细胞色素P450基因;KEGG(Kyoto encyclopedia of genes and genomes)分析发现淀粉和蔗糖代谢、戊糖和葡萄糖醛酸相互转化途径中糖苷水解酶、UDPG脱氢酶等基因上调表达。通过搜索转录因子数据筛选到172个差异表达的转录因子,预测了可能与漆酶结合的bZIP、C2H2、C4转录因子家族。由此推测,在漆酶高产单核菌株中木质素降解和碳水化合物代谢的相关基因的表达发生变化,及糖醛酸和磷酸戊糖途径相关基因上调表达,促进了木质素降解产物高效转化成糖、核酸等生物大分子,有助于香菇菌丝体的生长,转录因子在漆酶活性调控中起了重要作用。本研究为深入理解香菇漆酶高产菌株的生理代谢机制提供了重要的基因数据资源。  相似文献   

11.
The complete genome sequence of the Xanthomonas campestris pv. campestris strain B100 was established. It consisted of a chromosome of 5,079,003bp, with 4471 protein-coding genes and 62 RNA genes. Comparative genomics showed that the genes required for the synthesis of xanthan and xanthan precursors were highly conserved among three sequenced X. campestris pv. campestris genomes, but differed noticeably when compared to the remaining four Xanthomonas genomes available. For the xanthan biosynthesis genes gumB and gumK earlier translational starts were proposed, while gumI and gumL turned out to be unique with no homologues beyond the Xanthomonas genomes sequenced. From the genomic data the biosynthesis pathways for the production of the exopolysaccharide xanthan could be elucidated. The first step of this process is the uptake of sugars serving as carbon and energy sources wherefore genes for 15 carbohydrate import systems could be identified. Metabolic pathways playing a role for xanthan biosynthesis could be deduced from the annotated genome. These reconstructed pathways concerned the storage and metabolization of the imported sugars. The recognized sugar utilization pathways included the Entner-Doudoroff and the pentose phosphate pathway as well as the Embden-Meyerhof pathway (glycolysis). The reconstruction indicated that the nucleotide sugar precursors for xanthan can be converted from intermediates of the pentose phosphate pathway, some of which are also intermediates of glycolysis or the Entner-Doudoroff pathway. Xanthan biosynthesis requires in particular the nucleotide sugars UDP-glucose, UDP-glucuronate, and GDP-mannose, from which xanthan repeat units are built under the control of the gum genes. The updated genome annotation data allowed reconsidering and refining the mechanistic model for xanthan biosynthesis.  相似文献   

12.
【目的】Pseudomonas boreopolis GO2可以利用木质纤维素类生物质为唯一碳源发酵产微生物絮凝剂。解析菌株GO2的全基因组特征可为利用木质纤维素类生物质定向合成多糖型微生物絮凝剂提供分子基础。【方法】利用Illumina NovaSeq测序平台对菌株GO2进行测序,用SMRT等软件进行基因组组装、系统发育分析、基因预测和功能注释,并与4株近缘模式株进行了比较基因组分析。【结果】菌株GO2基因组大小为4 498 896 bp,GC含量为69.5%,共编码3 906个基因。菌株GO2与Pseudomonas boreopolis JCM 13306的16S r RNA基因相似性、平均核苷酸一致性(average nucleotide identity, ANI)、DNA-DNA杂交(DNA-DNA hybridization, DDH)值最高,分别为99.93%、98.36%和88.00%,将菌株GO2命名为Pseudomonas boreopolis GO2。比较基因组分析发现,GO2与4个近缘模式菌株共有2 348个直系同源核心基因,主要参与碳水化合物代谢、氨基酸代谢...  相似文献   

13.
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14.
Twelve genes coding for assembly, acetylation, pyruvylation, polymerization, and secretion of the polysaccharide xanthan gum are clustered together on the chromosome of the bacterium Xanthomonas campestris. These genes (gumBCDEFGHIJKLM) are sufficient for synthesis of xanthan gum when placed in bacteria from a different genus, Sphingomonas. The polysaccharide from the recombinant microorganism is largely indistinguishable, structurally and functionally, from native xanthan gum. These results demonstrate that a complex pathway for biosynthesis of a specific polysaccharide can be acquired by a single inter-generic transfer of genes between bacteria. This suggests the biological and commercial feasibility of synthesizing xanthan gum or other polysaccharides in non-native hosts. Received 23 October 1996/ Accepted in revised form 14 April 1997  相似文献   

15.
AIMS: Isolation and characterization of the xanthan-degrading Microbacterium sp. XT11. METHODS AND RESULTS: The bacterial isolate XT11, capable of fragmenting xanthan, has been isolated from soil sample. Morphological and biochemical analyses, as well as 16S rRNA gene sequence comparisons, demonstrated that strain XT11 should be grouped in the genus Microbacterium, and represented a new member in this family. Xanthan could be degraded by the xanthan-degrading enzyme released from strain XT11. It has been shown that xantho-oligosaccharides fragmented from xanthan had both elicitor activity and antibacterial effect against Xanthomonas campestris pv. campestris. CONCLUSIONS: The xanthan-degrading enzyme produced by the newly isolated XT11 could fragment xanthan to form oligosaccharides. SIGNIFICANCE AND IMPACT OF THE STUDY: Xanthan-degrading products would be useful for potential application in the control of black rot of cruciferous plants caused by X. campestris pv. campestris and, as an oligosaccharide elicitor, in making these plants resistant to disease.  相似文献   

16.
Lysine metabolism plays an important role in the formation of the insecticidal crystal proteins of Bacillus thuringiensis (Bt). The genes lam, gabD and sucA encode three key enzymes of the lysine metabolic pathway in Bt4.0718. The lam gene mainly affects the cell growth at stable period, negligibly affected sporulation and insecticidal crystal protein (ICP) production. While, the deletion mutant strains of the gabD and sucA genes showed that the growth, sporulation and crystal protein formation were inhibited, cells became slender, and insecticidal activity was significantly reduced. iTRAQ proteomics and qRT-PCR used to analyse the differentially expressed protein (DEP) between the two mutant strains and the wild type strain. The functions of DEPs were visualized and statistically classified, which affect bacterial growth and metabolism by regulating biological metabolism pathways: the major carbon metabolism pathways, amino acid metabolism, oxidative phosphorylation pathways, nucleic acid metabolism, fatty acid synthesis and peptidoglycan synthesis. The gabD and sucA genes in lysine metabolic pathway are closely related to the sporulation and crystal proteins formation. The effects of DEPs and functional genes on basic cellular metabolic pathways were studied to provide new strategies for the construction of highly virulent insecticidal strains, the targeted transformation of functional genes.  相似文献   

17.
Origins of the 2,4-dinitrotoluene pathway   总被引:6,自引:0,他引:6       下载免费PDF全文
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