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1.
Jin He Xiaohu Shao Huajun Zheng Mingshun Li Jieping Wang Qingye Zhang Lin Li Ziduo Liu Ming Sun Shengyue Wang Ziniu Yu 《Journal of bacteriology》2010,192(15):4074-4075
Bacillus thuringiensis has been widely used as a biopesticide for a long time. Here we report the finished and annotated genome sequence of B. thuringiensis mutant strain BMB171, an acrystalliferous mutant strain with a high transformation frequency obtained and stocked in our laboratory.Bacillus thuringiensis is an insect pathogen which is widely used as a biopesticide due to its various endogenous crystal proteins and spores (12). To improve the virulence and practical effectiveness of B. thuringiensis, genetic transformation of different genes with beneficial traits is a fundamental procedure. Simultaneously, genetic transformation can facilitate functional genomic research. However, wild-type strains are not suitable to be used as recipient strains because of low transformation efficiency. This obstacle is mainly caused by the thick cell wall layer of B. thuringiensis together with multiple plasmids inside the cell, which harbor genes encoding insecticidal crystal proteins. We used the method of elevating the growth temperature and adding 0.05% sodium dodecyl sulfate to treat several parental strains and finally obtained mutant strain BMB171, with no resident plasmid, from wild-type crystalliferous strain YBT-1463 (9). The electrotransformation frequency of mutant BMB171 could reach up to 107 transformants/μg DNA after optimization of the electrotransformation parameters (7), which was 4.8 × 104-fold higher than that of the parental strain (8). Moreover, mutant strain BMB171 exhibited the same characteristics as YBT-1463, such as metabolic abilities and growth properties, as well as sensitivity to 10 antibiotics (8). Of course, BMB171 could produce parasporal crystals with characteristic geometric shapes through the expression of relevant cry genes carried by plasmids (7). Thus, B. thuringiensis mutant strain BMB171 has become a major recipient strain and is widely used for insecticidal crystal protein-encoding gene expression (14, 15), cell surface display (10, 13), gene function and regulation researches (2, 5), etc.The B. thuringiensis mutant strain BMB171 genome was sequenced by using a massive parallel pyrosequencing technology (454 GS-FLX). A total of 448,963 high-quality reads with an average read length of 391 bp were produced, providing about 32-fold coverage of the genome. Assembly was performed using the Newbler software of the 454 suite package (454 Life Sciences), which resulted in 193 large (defined as >500 bp) contigs. The relationship of contigs was determined by multiplex PCR, and gaps were filled through sequencing of PCR products by primer walking or shotgun sequencing with an ABI 3730 sequencer. The Phred/Phrap/Consed software package (3) was used for final sequence assembly and quality assessment. Protein-coding genes were predicted by combining the results of Glimmer 3.02 (1) and ZCURVE (4), followed by manual inspection. Both tRNA and rRNA genes were identified by tRNAscan-SE (11) and RNAmmer (6), respectively. Functional annotation was performed by searching against a protein database of the microbial genome developed in house.The 5.64-Mb genome of B. thuringiensis mutant strain BMB171 contains two replicons: a circular chromosome (5.33 Mb) encoding 5,088 open reading frames (ORFs) and a circular plasmid (0.31 Mb), which is named pBMB171, encoding 276 predicted ORFs. The G+C content of the chromosome is 35.3%, while that of the plasmid is 33.3%. The mutant strain BMB171 genome encodes 104 tRNAs and 14 rRNA operons. A previous study indicated that BMB171 is a plasmid-free mutant (9); however, our sequencing results demonstrated that a large plasmid still remains. The reason why the plasmid was not detected previously might be its large size and low copy number. We did not find any crystal protein genes in either chromosome or plasmid sequences, which was consistent with previous observations (9).In summary, the complete B. thuringiensis mutant strain BMB171 genome provides a better-defined genetic background for gene expression and regulation studies, especially crystal protein production and metabolic network construction. 相似文献
2.
Peng Guan Peng Ai Xiaojuan Dai Jing Zhang Lizhi Xu Jun Zhu Qiao Li Qiming Deng Shuangcheng Li Shiquan Wang Huannian Liu Lingxia Wang Ping Li Aiping Zheng 《Journal of bacteriology》2012,194(24):6975
Bacillus thuringiensis is an important microbial insecticide used in the control of agricultural pests. Here we report the finished, annotated genome sequence of Bacillus thuringiensis serovar Sichuansis strain MC28, which can form parasporal crystals consisting of Cry4Cc1, Cry30Fa1, Cry53Ab1, Cry54Aa1, Cry54Ab1, Cry68Aa1, Cry69Aa1, Cry69Aa2, Cry70Ba1, Cyt1Da1, and Cyt2Aa3. It is also highly toxic to lepidopterous and dipterous insects. 相似文献
3.
Alcanivorax dieselolei B5T was isolated from oil-contaminated surface water of the Bohai Sea of China and characterized by the efficient degradation of alkane (C5-C36). Here we report the complete genome of B5T and genes associated with alkane degradation. 相似文献
4.
Satoru Watanabe Yuh Shiwa Mitsuhiro Itaya Hirofumi Yoshikawa 《Journal of bacteriology》2012,194(24):7007
Genome synthesis of existing or designed genomes is made feasible by the first successful cloning of a cyanobacterium, Synechocystis PCC6803, in Gram-positive, endospore-forming Bacillus subtilis. Whole-genome sequence analysis of the isolate and parental B. subtilis strains provides clues for identifying single nucleotide polymorphisms (SNPs) in the 2 complete bacterial genomes in one cell. 相似文献
5.
Guangjun Gao Jing Li Tiefeng Li Zhengfang Zhang Liping Wang Xitong Yuan Yufei Wang Jie Xu Yuehua Ke Liuyu Huang Dali Wang Zeliang Chen Xingran Xu 《Journal of bacteriology》2012,194(23):6680
Brucella canis infects several species of animals, and canine is the preferred host. Genome sequences of strains from different hosts are valuable for comparative analysis of host adaptation and microevolution. Here, we report the genome sequence of Brucella canis strain 118, a strain isolated from canine. 相似文献
6.
Yoshiyuki Ohtsubo Fumito Maruyama Hisayuki Mitsui Yuji Nagata Masataka Tsuda 《Journal of bacteriology》2012,194(24):6970-6971
We report the complete genome sequence of Acidovorax sp. strain KKS102, a polychlorinated-biphenyl-degrading strain isolated from a soil sample in Tokyo. The genome contains a single circular 5,196,935-bp chromosome and no plasmids. 相似文献
7.
Complete Genome Sequence of the Extremophilic Bacillus cereus Strain Q1 with Industrial Applications
Zhaohui Xiong Yan Jiang Danhua Qi Huaibao Lu Fan Yang Jian Yang Lihong Chen Lilian Sun Xingye Xu Ying Xue Yafang Zhu Qi Jin 《Journal of bacteriology》2009,191(3):1120-1121
Bacillus cereus strain Q1 was isolated from a deep-subsurface oil reservoir in the Daqing oil field in northeastern China. This strain is able to produce biosurfactants and to survive in extreme environments. Here we report the finished and annotated genome sequence of this organism.Bacillus cereus strain Q1 was isolated from a deep-subsurface oil reservoir in the Daqing oil field in northeastern China. This strain can facilitate oil recovery when added to an oil reservoir. This attribute may be partially due to its ability to produce biosurfactants, which assist microbial enhanced oil recovery by lowering interfacial tension at the oil-rock interface (data not shown).The complete genome sequence of B. cereus Q1 was determined by the whole-genome shotgun strategy. Draft assemblies were based on 55,790 high-quality reads. All libraries provided sixfold coverage of the genome. Gap closure was accomplished by primer walking on gap-spanning clones and direct sequencing of combinatorial PCR products. Open reading frame (ORF) predictions were obtained and annotation was performed as described previously (4). GenomeComp was used for genomic comparison with default parameters (5).The genome of B. cereus Q1 is composed of one circular chromosome of 5,214,195 bp and two circular plasmids (pBc239 [239,246 bp] and pBc53 [52,766 bp]) with mean G+C contents of 35.6, 33.5, and 35.1%, respectively. There are 5,657 predicted ORFs, 13 rRNA operons, and 94 tRNA genes for all 20 amino acids, covering 86% of the genome. Putative functions were assigned to 3,946 ORFs. Of the remainder, 1,561 showed similarity to hypothetical proteins and 140 had no detectable homologs in the public protein database (E value, <10−10). Twelve phage-related genes were identified, but no complete prophages were found. Whole-genome comparison showed that Q1 has extensive similarity to the genomes of other members of the B. cereus group and the greatest similarity to nonpathogenic strain B. cereus ATCC 10987 (5,224,283 bp).Genome analysis revealed that B. cereus Q1 contains several genes related to niche-specific adaptations. As a thermophilic bacterium, Q1 can easily adapt to geothermal oil reservoirs. Three thermophily-associated genes (BC1015, BC1017, and BC1018) found in Q1 have orthologs in Moorella thermoacetica ATCC 39073. The latter genes encode the structural maintenance of chromosome protein, exonuclease SbcC, and subunit A of DNA topoisomerase VI, respectively. The presence of the genes involved in the utilization of l-fucose (BC2995 to BC3006) and d-mannose (BC5091 to BC5094, BC5097 to BC5102, and BC5105 to BC5111) helps Q1 use these carbohydrates as carbon sources under glucose-limited conditions. Q1 also contains the nitrate utilization gene cluster (BC2100 to BC2123), including a typical narGHJI operon that encodes membrane-bound nitrate reductase. The nitrate utilization gene cluster might play an important role in helping the strain use nitrate as a nitrogen source and survive under anaerobic or oxygen-limited conditions. Moreover, we found an operon that encodes proteins responsible for producing a novel type of lantibiotic (2), which we designated cereicidin. All of the above-mentioned genes were not found in the other B. cereus group bacteria.One of the notable features of Q1 is its ability to produce biosurfactants. The dhb operon (dhbACEBF), which is involved in nonribosomal peptide synthesis and encodes the biosynthetic template for the catecholic siderophore in B. subtilis (1), was identified in Q1. Downstream of the operon, the sfp gene, which encodes phosphopantetheinyl transferase and is required for production of the lipopeptide antibiotic surfactin in B. subtilis (3), was found. No surfactin synthetase gene (srfAA, srfAB, or srfAC) was found, but the mbtH gene involved in mycobactin synthesis and a gene (BC2300) with an unknown function were found in the region between the dhb operon and the sfp gene. We therefore speculated that these three genes located downstream of the dhbF gene might belong to the dhb operon, which is involved in antibiotic-siderophore-surfactin biosynthesis.The B. cereus Q1 genome provides an excellent platform for the further improvement of this organism for biosurfactant production and extends our understanding of the evolutionary relationships among B. cereus group organisms. 相似文献
8.
AP Dos Santos AM Guimaraes NC do Nascimento PJ Sanmiguel JB Messick 《Journal of bacteriology》2012,194(19):5458-5459
Mycoplasma wenyonii is a hemotrophic mycoplasma that causes acute and chronic infections in cattle. Here, we announce the first complete genome sequence of this organism. The genome is a single circular chromosome with 650,228 bp and G+C% of 33.9. Analyses of M. wenyonii genome will provide insights into its biology. 相似文献
9.
Streptococcus mutans, a principal causative agent of dental caries, is considered to be the most cariogenic among all oral streptococci. Of the four S. mutans serotypes (c, e, f, and k), serotype c strains predominate in the oral cavity. Here, we present the complete genome sequence of S. mutans GS-5, a serotype c strain originally isolated from human carious lesions, which is extensively used as a laboratory strain worldwide. 相似文献
10.
Thomas A. Tompkins Guillaume Barreau Jeffery R. Broadbent 《Journal of bacteriology》2012,194(22):6349
Lactobacillus helveticus R0052 is a commercially available strain that is widely used in probiotic preparations. The genome sequence consisted of 2,129,425 bases. Comparative analysis showed that it was unique among L. helveticus strains in that it contained genes encoding mucus-binding proteins similar to those found in Lactobacillus acidophilus. 相似文献
11.
新分离的副粘病毒Tianjin株的全基因组序列分析 总被引:2,自引:0,他引:2
副粘病毒Tianjin株是一株对普通棉耳狨猴具有高致病性,并可能与人类下呼吸道感染密切相关的毒株.为了明确其基因结构、变异特点及种系进化地位,采用RT PCR、测序和拼接,获得了副粘病毒Tianjin株全基因组序列,与GenBank登录的副粘病毒科7个属和尚未分类的28株病毒及7株仙台病毒代表株,进行同源性比较及系统进化分析.结果表明,副粘病Tianjin株属于副粘病毒科、副粘病毒亚科、呼吸道病毒属,与仙台病毒关系最近.基因组全长及组成规律与仙台病毒相似,只是L基因末尾A15240C变异而使L蛋白增加了一个谷氨酸残基.副粘病毒Tianjin株存在440个独特的核苷酸变异位点,导致110个氨基酸残基的改变,系统进化上构成独立的分支.副粘病毒Tianjin株在基因组序列、宿主亲嗜性和致病性等方面与已知仙台病毒存在较大的差异,可能代表仙台病毒的一个新基因型. 相似文献
12.
Wei Liu Liurong Fang Sha Li Qiang Li Zhemin Zhou Zhixin Feng Rui Luo Guoqing Shao Lei Wang Huanchun Chen Shaobo Xiao 《Journal of bacteriology》2010,192(21):5844-5845
Mycoplasma hyorhinis is generally considered a swine pathogen yet is most commonly found infecting laboratory cell lines. An increasing body of evidence suggests that chronic infections with M. hyorhinis may cause oncogenic transformation. Here, we announce the complete genome sequence of M. hyorhinis strain HUB-1.Mycoplasma hyorhinis is generally considered to be a swine pathogen causing lung lesions, inflammation in the chest and abdominal lining, and arthritis (8). This agent also frequently contaminates laboratory cell cultures, impinging on many aspects of biological research (3). Recent studies have demonstrated that M. hyorhinis infections induce a malignant phenotype in human prostate (7) and gastric (4) cells, suggesting that M. hyorhinis infections are associated with oncogenic transformation. These properties of M. hyorhinis have increased its profile to researchers. The complete genome sequence of this microbe has yet to be determined.We sequenced the genome of M. hyorhinis strain HUB-1, a pathogenic strain isolated from the respiratory tract of swine. Whole-genome sequencing was performed by combining GS FLX (6) and Solexa paired-end sequencing technologies (1). Genomic libraries containing 3-kb inserts were constructed, and 308,604 reads (79.7% paired end) were produced using the GS FLX system, giving 65.9-fold coverage of the genome. About 93.4% of reads were assembled into one large scaffold using Newbler software (454 Life Sciences, Branford, CT). A total of 822,579 reads were generated using an Illumina Solexa Genome Analyzer IIx and were mapped to the scaffold using the Burrows-Wheeler alignment (BWA) tool (5). Gaps were filled by local assembly of the Solexa/Roche 454 reads or by sequencing PCR products by using an ABI 3730 capillary sequencer. Open reading frames containing more than 30 amino acid residues were predicted using Glimmer 3.0 (2) and verified by comparison with six other closely related genome sequences.The complete genome of M. hyorhinis HUB-1 consists of an 839,615-bp single circular chromosome with an average G+C content of 25.88%. A total of 654 protein-encoding genes are predicted. The average protein size is 364 amino acids, and the mean coding percentage is 85.2%. The genome includes 30 tRNA genes, and only a single copy of the 16S-23S rRNA operon can be found. The 5S rRNA operon is separate from the 16S-23S rRNA operon. Protein secretion occurs through a truncated membrane protein secretion system, consisting of SecA, SecD, SecY, PrsA, DnaK, Tig, and LepA. Additionally, 20 pseudogenes, which become truncated or inactivated, are identified in the genome.M. hyorhinis contains a special variable lipoprotein (Vlp) system that constitutes its major coat protein (9) and provides a mutational strategy for evasion of the host immune system. Different M. hyorhinis strains carry a variable number of vlp genes (9). M. hyorhinis HUB-1 is characterized to contain seven vlp genes displayed in the order 5′-vlpD-vlpE-vlpF-insertion sequence (IS)-vlpG-vlpA-IS-vlpB-vlpC-3′.This is the first complete genome sequence of M. hyorhinis, and its availability will provide a better-defined genetic background for future studies of gene expression and regulation. 相似文献
13.
Streptococcus thermophilus MN-ZLW-002 was originally isolated from traditionally fermented Chinese dairy products. One of the strain-dependent characteristics of this bacterium is its ability to produce exopolysaccharides (EPSs). This study determined and analyzed the genome sequence of MN-ZLW-002. Its complete genome comprised 2,046 genes and 1,848,520 nucleotides with an average GC content of 39%. The EPS cluster of MN-ZLW-002 includes 25 open reading frames (ORFs), and some results indicate a horizontal gene transfer between MN-ZLW-002 and other lactic acid bacteria (LAB). 相似文献
14.
Here we announce the complete genome sequence of the coenzyme B(12)-producing enteric bacterium Shimwellia blattae (formerly Escherichia blattae). The genome consists of a single chromosome (4,158,636 bp). The genome size is smaller than that of most other enteric bacteria. Genome comparison revealed significant differences from the Escherichia coli genome. 相似文献
15.
Ann-Chi Lin Tsai-Lien Liao Yi-Chun Lin Yi-Chyi Lai Min-Chi Lu Ying-Tsong Chen 《Journal of bacteriology》2012,194(22):6316
We report the complete genome sequence of Klebsiella pneumoniae 1084, a hypermucoviscosity-negative K1 clinical strain. Sequencing and annotation revealed a 5,386,705-bp circular chromosome (57.4% G+C content), which contains 4,962 protein-coding genes, 80 tRNA genes, and 25 rRNA genes. 相似文献
16.
The genus Acinetobacter is ubiquitous in soil, aquatic, and sediment environments and includes pathogenic strains, such as A. baumannii. Many Acinetobacter species isolated from various environments have biotechnological potential since they are capable of degrading a variety of pollutants. Acinetobacter sp. strain DR1 has been identified as a diesel degrader. Here we report the complete genome sequence of Acinetobacter sp. DR1 isolated from the soil of a rice paddy.The genus Acinetobacter appears to be metabolically versatile and has the ability to degrade aliphatic hydrocarbon, thus making it an organism of interest for its possible bioremediational potential (9). Despite its biotechnological potential, the majority of genome projects conducted with Acinetobacter species have focused on pathogenic strains of A. baumannii. Currently, the only available whole-genome sequence of environmental isolates is that of A. baylyi ADP1 (2). Acinetobacter sp. strain DR1 was isolated from the soil of rice paddies, located in Deok-So (Korea University Agricultural Station), in the Kyonggi province of South Korea. Strain DR1 is capable of utilizing aliphatic hydrocarbons and diesel oil (5). Similarly to A. baylyi ADP1, this strain is also competent for natural transformation. We demonstrated previously that sodium chloride added to the medium induces the overproduction of exopolysaccharide (EPS), which evidences protective activity against diesel toxicity (4). Interestingly, DR1 possesses a quorum sensing (QS) system, which has been shown to play a significant role in biofilm formation and hexadecane biodegradation. The results of proteomic studies have demonstrated that the QS system regulates a broad variety of proteins (6). Collectively, our findings demonstrate that DR1 has profound potential for environmental applications and is an environmental isolate distinct from pathogenic strains, thus indicating that the whole-genome sequencing of DR1 is a worthwhile pursuit.Initial pyrosequencing using a GS-FLX system (454 Life Science Corporation) generated 652,162 reads (264,482,836 nucleotides; 64.3-fold coverage), which were assembled into 56 contigs. To determine the order of the contigs, 1,248 fosmid clones were constructed with an average insert size of 35 kb (10.5-fold coverage). The fosmid-end sequencing of 936 clones generated 1,372,452 bp. These high-quality Sanger reads allowed the assembly of 41 large contigs into 2 scaffolds containing 38 gaps. The gaps were filled via primer walking. All procedures for genome sequencing and gap filling were conducted by Macrogen (Seoul, South Korea). Protein coding regions were predicted with the GLIMMER3 software program (3), and automatic genome annotation was conducted on a RAST server (1) and the NCBI Prokaryotic Genomes Automatic Annotation Pipeline (PGAAP). The tRNA and rRNA genes were annotated using the tRNAScan-SE (8) and RNAmmer software programs (7), respectively. The genome of Acinetobacter sp. DR1 consists of a circular 4,152,543-bp chromosome with a G+C content of 38%, 3,874 predicted coding sequences, and 71 tRNAs. There are 6 rRNA operons with a 16S, tRNA-Ile, tRNA-Ala, 23S, 5S organization. The genes studied previously were clearly identified via genome sequencing (4, 5, 6). The availability of the complete genome sequence of Acinetobacter sp. strain DR1 will contribute to an in-depth understanding of the genetic potentials of Acinetobacter species. 相似文献
17.
Yu Xue Qingmei Xie Zhuanqiang Yan Jun Ji Feng Chen Jianping Qin Baoli Sun Jingyun Ma Yingzuo Bi 《Journal of virology》2012,86(24):13812-13813
Recently, nephropathogenic infectious bronchitis virus (IBV) outbreaks have occurred in commercial broiler flocks and have been associated with a high incidence and morbidity in China. The CK/CH/Zhejiang/06/10 strain (IBV-YX10) was isolated from a 12-day-old broiler chicken in a flock of chickens with swollen speckled kidneys and distended ureters filled with uric acid in China in 2010. Here we reported the complete genomic sequence of the IBV-YX10 which was a natural recombinant nephropathogenic infectious bronchitis virus strain. These findings will contribute additional insights into the molecular characteristics of evolving IBV genomes and the need for effective control of IBV in China. 相似文献
18.
Feng Chen Yongfei Pan Chengqiu Liao Qingfeng Zhou Xiangbin Zhang Yanhua Song Yingzuo Bi 《Journal of virology》2012,86(22):12457-12458
Porcine circovirus type 2 (PCV2) is the etiologic agent of porcine circovirus-associated disease, and it is mainly divided into five genotypes. Here, we report the complete genome sequence of PCV2 strain GDYX, which belongs to PCV2d and has a unique amino acid variation at position 169 (S to G). 相似文献
19.
Shaojian Xu Jun Li Xiaoyuan Yuan Guisheng Wang Jianli Shi Jiaqiang Wu Xiaoyan Cong Wenbo Sun Yijun Du Tongjie Chai Jinbao Wang 《Journal of virology》2012,86(24):13885
Shandong is a porcine circovirus 2b (PCV2b) strain that was isolated and purified from tissue samples from pigs with postweaning multisystemic wasting syndrome (PMWS) in the Shandong Province of China. Here, we report the complete genome sequence of strain Shandong, which may aid in understanding the molecular characteristics of this strain. 相似文献
20.
Yung S. Ho Sabir A. Adroub Maram Abadi Bader Al Alwan Reham Alkhateeb Ge Gao Alaa Ragab Shahjahan Ali Dick van Soolingen Wilbert Bitter Arnab Pain Abdallah M. Abdallah 《Journal of bacteriology》2012,194(22):6339-6340
Mycobacterium vaccae is a rapidly growing, nontuberculous Mycobacterium species that is generally not considered a human pathogen and is of major pharmaceutical interest as an immunotherapeutic agent. We report here the annotated genome sequence of the M. vaccae type strain, ATCC 25954. 相似文献