人源H3N2亚型猪流感重组病毒的分离鉴定及全基因序列分析

本研究由疑似猪流感病料样品中分离一株病毒,通过HA、HI、电镜观察、生物学特性测定及全基因序列测定表明,分离病毒株为H3N2亚型人流感病毒和H1N1亚型古典猪流感病毒(SIV)的重组体,命名为A/Swine/Fujian/F2/07(H3N2).该分离株含有8个基因片段,共13 442 bp,与GenBank中登录的H3N2亚型人流感病毒、H1N1亚型古典SIV和H3N2亚型SIV进行比较分析显示:分离株的HA、NS、NA基因与H3N2亚型人流感病毒株的同源性分别为84.7 ％～98.1％、94.4 ％～99.5％和88.6 ％～97.6％;与H3N2亚型SIV的核苷酸同源性分别为87.7％～98.5％、82.5 ％～99.9％和87.6 ％～98.4％;M基因与H3N2亚型人流感病毒和SIV的同源性均在90.1％以下,而与H1N1亚型古典SIV的同源性在97.6％以上.基因型分析表明分离株的PB2、PBI、PA、HA、NP、NA和NS基因片段来源于1975年～1982年的人流感病毒,而M基因来源于H1N1亚型古典SIV,充分证明猪作为流感病毒“混合器”的作用.     

猪瘟病毒石门株基因组cDNA片断的扩增与克隆测序

以猪瘟病毒（ＨＣＶ）中国石门株强毒的血毒、细胞毒及Ｃ系兔化弱毒的细胞毒中提取的总ＲＮＡ为模板，应用逆转录─聚合酶链式反应（ＲＴ一ＰＣＲ），在合成的两对ＨＣＶ特异引物引导下，扩增出与预计大小一致的４４１和３００ｂｐ两个核酸片断。寡核苷酸探针杂交证实确为ＨＣＶＰ_８０和ｇｐ４４／４８蛋白编码区特异性的ｃＤＮＡ片断。扩增片断克隆入ｐＵＣ_１９和ｐＢＳＫ（＋）中，并对ＨＣＶ石门株Ｐ_８０区ｃＤＮＡ片断进行测序分析，其与国外Ａｌｆｏｒｔ、Ｂｒｅｓｃｉａ株同源性分别为９０．６％和９４．６％。氨基酸水平上同源性高达９８．４％。为抗猪瘟病毒Ｐ_８０区核酶的设计和应用提供了依据。     

驯鹿18S rRNA基因的克隆测序

对驯鹿 (Rangifertarandus)的 1 8SrRNA基因片段进行了克隆测序 ,序列长度为 1 1 47bp ,并且已被发送到Genebank上 ,其登录号是AY1 45 5 2 7。     

The Application of Microbiome Culturomics in Veterinary Medicine

Under laboratory conditions, the number of cultured microorganisms accounts for about 1% of the total number of microorganisms in nature, which limits people's understanding and utilization of 99% of the unknown microorganisms. However, relevant researches show that those "uncultured microorganisms" can be developed and utilized, and the uncultured microorganisms are the main body of the unknown microorganisms. The microbial culturomics explored the application of multiple culture conditions and long-term culture, it was combined with Matrix-Assisted Laser Desorption/Ionization Time of Flight Mass Spectrometry (MALDI-TOF-MS) and 16S ribosomal RNA (rRNA) sequencing to identify all kinds of microorganisms on a large scale. At the same time, whole-genome sequencing (WGS) and Metagenomics sequencing technology were used to analyze unknown microorganisms in depth. In this paper, the latest progress of culturomics in the ruminant gastrointestinal tract, poultry cecum, and livestock nasal microflora in recent years was reviewed, and the feasibility of applying the method of microflora culturomics in animal disease prevention and control was discussed. As a new research idea, culturomics has some immature aspects, but its development prospect is very broad. The complementary of microflora culturomics and other research methods have gradually become a breakthrough in the development of veterinary microbiology.     

High Throughput Sequencing to Study the Effect of Chronic Renal Failure on the Diversity and Gene Function Prediction of Gut Microbiota in Dogs

This study aimed to investigate the effect of chronic renal failure(CRF) on the gut microbiota diversity and predict the gene function of the flora. A total of 30 2-year-old dogs were selected and randomly divided into the chronic renal failure model group (CRF, established by renal artery ligation), sham operation control group (Sham) and healthy control group (HCG). All animals were fed normally during the 56 days of test period. The serum creatinine (Scr), blood urea nitrogen (BUN) and urine protein / creatinine ratio (UP/C) were detected regularly during the experiment. The effects of chronic renal failure on the structure, diversity and function of gut microbiota were analyzed according to the result of bacterial 16S rDNA sequencing from fresh feces collected without contamination. The flora markers index (FMI) was constructed based on the principal component Logistic regression analysis of different microbiota in CRF group to predict the development of chronic renal failure. The results showed that: 1) The levels of Scr, BUN and UP/C in CRF group from the start of the 28th day of the experiment were significantly higher than those of HCG group and Sham group (P<0.05), and significantly higher than that of the first day of CRF group (P<0.05). 2) Compared with those before chronic renal failure (CRF group at day 0 and 28), HCG group and Sham group, the Chao 1 diversity and Shannon diversity of gut microbiota in CRF group at day 56 were significantly lower (P<0.05), while the relative abundance of Bacteroidetes, Proteobacteria and Actinobacteria significantly increased and the number of Firmicutes significantly decreased (P<0.05). 3) LEfSe analysis showed that 20 species were enriched in CRF group, mainly including Pseudomonas, Escherichia, Proteus and so on, and most of them had negative correlation with other intestinal bacteria. Functional prediction revealed that genes of those different species were mainly enriched in amino acid metabolism, sugar biosynthesis and metabolism and carbohydrate metabolism in CRF group. The area under ROC curve (AUC) of the FMI constructed with those species enriched was 0.788, which could be used as the intestinal microbial marker for CRF in dogs. In summary, chronic renal failure can reduce the diversity of intestinal microbiota, lead to the imbalance of bacterial structure and change of bacterial function. Moreover, the enriched gut microbiota in CRF group can be used as the intestinal microbial marker of CRF in dogs, and the best prediction effect can be obtained by FMI.     

基因组测序技术解析耐除草剂转基因水稻G2-7的分子特征

Molecular characterization, such as copy number and flanking sequence of foreign DNA fragment insertion site, is the important identity information, provided during safety assessment of genetic modified crop. In this study, the T-DNA insertion site, copy number and flanking sequences were identified in transgenic glyphosate-tolerant rice G2-7 based on whole genome sequencing in combination bioinformatics analysis method. 47.13 Gb clean sequence data for G2-7 was generated on Illumina NovaSeq 6000 platform. The junction reads mapped to boundaries of T-DNA and flanking sequences in G2-7 were identified by comparing with sequence of transformation vector and rice reference genome. The results showed that exogenous T-DNA fragments was integrated in the position of Chr. 1 36,189,491-36,189,507 with a single copy, 16 bp rice genome sequence was deleted at the insertion site and no insertion of vector backbone. 375 bp and 353 bp flanking host DNA sequence of 5′-end and 3′-end of the insertion DNA fragment were also obtained, respectively. The putative insertion location and flanking sequences were further confirmed by PCR amplification and Sanger sequencing. The results not only provided data support for safety assessment and event specific detection, but also demonstrated that WGS was an effective technique for identifying molecular characterization in rice.     

犬巴贝西虫病PCR检测方法的建立

为快速、准确检测犬巴贝西虫病,根据GenBank中收录的犬的巴贝西虫18sRNA基因序列,设计合成1对特异性诊断引物,建立了PCR诊断方法。结果扩增出了犬巴贝西虫18sRNA基因的一段大小为319bp片段,经测序,所扩增序列与报道的序列完全匹配。同时对附红细胞体、巴氏杆菌DNA样品进行扩增没有出现扩增条带。阳性犬全血DNA稀释1 000倍后,依然可以有效地检测出虫体DNA。结果表明,所建立的PCR检测方法,具有极高的敏感性和特异性,可以运用于临床检测巴贝西虫病。     

鸭瘟病毒河南株gI基因的克隆与测序

参考GenBank中鸭瘟病毒gI基因序列设计并合成引物,以鸭瘟病毒河南分离株DNA为模板进行PCR扩增,将扩增片段克隆至PGEM-T载体上,得到含gI基因重组质粒。经酶切鉴定,并对重组阳性质粒进行序列测定。结果表明,获得的片段含鸭瘟病毒gI基因,全长1 089 bp,与已报道的其他疱疹病毒gI基因具有较高的同源性,编码432个氨基酸,蛋白分子质量为39.7ku、等电点(PI)为6.06。