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本研究利用RT-PCR结合RACE技术,从感染柑橘叶斑驳病毒(Citrus leaf blotch virus, CLBV)的叶片中获得了江西分离物CLBV-JX的全基因组序列,并对其序列特征进行分析。CLBV-JX全长8747 nt,编码3个开放阅读框,序列一致性比较结果显示,与来源于柑橘的分离物序列一致度高,均大于95.9%以上,与甜樱桃和猕猴桃来源的分离物序列一致性低,3"端非编码区的核酸一致性仅为62.7%和62.7%。系统进化分析中,CLBV-JX与所有柑橘来源分离物聚为一支,表现出较近的亲缘关系,与其他寄主来源分离物亲缘关系远。推测CLBV的遗传分化可能与寄主存在一定的相关性。 相似文献
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猪CTSD全长cDNA的克隆和表达分析 总被引:1,自引:0,他引:1
以人CTSD mRNA全长序列为基序,在db EST库中搜索同源性大于80%、重叠大于40个碱基的猪EST下载经Seqman软件装配后,利用RT-PCR扩增到猪CTSD基因部分cDNA序列,进一步通过RACE技术获得cDNA全长(GenBank登录号为DQ018727),猪CTSD基因cDNA全长2032 bp包括93 bp 5′UTR区、706 bp 3′UTR区和1 233bp ORF,编码410个氨基酸残基。其编码区与人、鼠、牛、羊CTSD编码区同源性分别为87.9%、78.2%、86.6%和85.0%,其氨基酸序列与人、鼠、牛、羊氨基酸序列同源性分别为86.6%、80.1%、86.0%和84.7%。疏水性分析和信号肽预测发现猪CTSD氨基酸序列存在至少7个疏水性区域,信号肽位点为第1-20个氨基酸残基。在NCBI进行Blast P搜索结果显示猪CTSD氨基酸结构中含有Asn(Asparagine,天门冬酰胺)结构域,与天冬氨酸蛋白酶3D结构同源性高达99.7%,具有真核生物天冬氨酸蛋白酶的典型结构。以猪多组织RNA池为模板,以1026 bp部分cDNA序列作为杂交探针进行Northern杂交,得到一条2000 bp左右特异条带,从而验证了RACE产物为全长cDNA并揭示该基因只有一个转录本。为了研究猪CTSD基因在体内不同组织内表达的特点,采用半定量RT-PCR对CTSD基因在猪10个组织中的表达进行研究,结果表明在10个组织中均有表达,且表达量与-βactin内参接近。 相似文献
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通过RT-PCR和RACE方法克隆了山羊Hspb10基因cDNA序列并进行了序列分析。结果表明:山羊Hspb10 cDNA全长1 056 bp,编码区全长780 bp,共编码259个氨基酸,提交至GenBank数据库中,收录号为JX067553。用Clustal W方法比对不同物种氨基酸序列同源性,山羊Hspb10与牛的同源性最高,核苷酸和氨基酸序列相似性分别为93.4%和96.5%;编码氨基酸序列BLAST比对结果也表明,哺乳动物Hspb10氨基酸序列极为保守,与禽类差异较大。获得山羊Hspb10 cDNA序列,可以为分子水平上研究山羊Hspb10的生物学功能奠定基础。 相似文献
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参照GenBank登录的绵羊凝乳酶原前体cDNA序列设计引物,以新生5d的西农萨能羊皱胃组织总RNA为模版,通过RT-PCR方法获得凝乳酶原前体cDNA,克隆测序后进行序列比对。结果表明,克隆基因为B型凝乳酶,该基因cDNA具有1292个碱基,编码381个氨基酸,包含16个氨基酸的信号肽序列和42个氨基酸的酶原序列。将其与已报道的山羊、绵羊和牛的凝乳酶原前体序列进行比对,发现核苷酸同源性分别为99.41%、98.74%和95.29%,氨基酸同源性为99.21%、98.42%和93.70%。 相似文献
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夜来香花叶病毒(telosma mosaic virus, TeMV)是侵染西番莲的重要植物病毒之一。本研究通过RACE和RT-PCR技术获得3条TeMV江西分离物全基因组序列,除poly(A)尾外,3个分离物基因组全长均为10069 nt。试验中采用汁液摩擦接种的方式对分离物进行生物学特性研究,首次发现该病毒可侵染豌豆寄主。对所获分离物全基因组进行序列一致性分析,结果显示,江西分离物间核苷酸与氨基酸序列一致性分别为98.1%-98.6%和98.8%-99.3%,与GenBank中报道的TeMV分离物全基因组的核苷酸与氨基酸序列一致分别为87.3%-98.9%和91.2%-99.5%,其中与武夷山分离物(MK340755)序列一致性最高。基于不同分离物CP基因的系统发育分析显示,寄主来源相同的分离物亲缘关系较近,推测TeMV的遗传进化与不同的植物寄主相关。 相似文献
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为探究赣南地区柑橘黄龙病菌的遗传多样性。从赣南16个县市区采集32个具典型柑橘黄龙病症状的脐橙样品,运用PCR-RFLP(聚合酶链式反应-限制性长度多态性分析)技术研究了柑橘黄龙病菌16S rDNA序列、16S/23S rDNA间隔区序列和核糖体蛋白基因的遗传多态性;并对三个基因片段进行测序,分析其序列的碱基含量、转换与颠换、同源性、核苷酸遗传距离和系统进化特征。RFLP结果表明:赣南16个县市区柑橘黄龙病菌XbaⅠ酶切图谱均与亚洲韧皮部杆菌(Candidatus Liberibacter asiaticus, CLas)的一致;进一步分析显示,三个基因片段各自之间的RFLP指纹图谱一致,并未表现多态性。序列分析结果表明:32个分离物三个基因片段各自的同源性均在98%~100%,与CLas的同源性最大,且与CLas的遗传距离最小。系统进化树展示赣南地区柑橘黄龙病菌与CLas处于同一分支,结合酶切图谱、序列同源性及系统进化分析结果表明: 赣南地区柑橘黄龙病菌均为CLas。结论:赣南地区柑橘黄龙病菌的16S rDNA序列、16S/23S rDNA间隔区序列和核糖体蛋白基因未表现遗传多样性,表明赣南地区柑橘黄龙病菌间遗传多样性不显著。
关键词:柑橘黄龙病;16S rDNA序列;核糖体蛋白基因;16S/23S rDNA间隔区;RFLP;序列分析 相似文献
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研究旨在对猪T细胞诱导型刺激物(ICOS)基因的cDNA序列进行克隆与分析。根据已报道的人ICOS基因cDNA序列设计引物,首次从猪脾脏组织总RNA中扩增出ICOS基因编码区全长cDNA序列,克隆于pMD18-T载体后进行测序并进行序列拼接,运用生物信息学分析DNA序列。结果表明:该基因编码区全长630bp,编码210个氨基酸,包含5个外显子。该序列与人全基因核苷酸序列及推导的氨基酸序列的同源性分别为80%和85%;与狗和小鼠的推导氨基酸序列的同源性分别为81%和75%。这为进一步研究该基因的结构特点和功能奠定了良好基础。 相似文献
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根据GenBank中猪Ⅱ型圆环病毒(PCV-2)基因序列,设计两对特异性引物.将PCV-2广东分离株(GD1株)用PK15细胞系培养,从细胞培养物中提取病毒总DNA并以之为模板,用PCR方法分段扩增病毒全基因组,分别克隆到pMD18-T载体,对阳性质粒进行序列测定.用DNAstar对序列进行拼接,得到PCV-2 GD1株基因组全序列,全长为1767个碱基,包涵2个开放阅读杠(ORF1和ORF2),分别编码与复制相关的Rep蛋白和结构蛋白Cap.通过BLAST对所测GD1株核苷核酸序列早国内外已登录GenBank中的PCV-2病毒核苷酸序更进行同源性比较,与PCV-2参考毒株的核苷酸同源性介于94.4%~99.7%之间,与德国株PCV-2(AF201897)的同源性最高,为99.7%;与猪I型圆环病毒(PCV-1)参考株(AY184287)的同源性仅为70%. 相似文献
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通过反转录-聚合酶链反应(RT-PCR),从中国北京分离株牛流行热病毒JB76H基因组RBA中扩增出主要保护性抗原糖蛋白G的cDNA。采用Sanger’s双脱氧末端终 止法测定cDNA片段的核苷酸序列,并推导出氨基酸序列。G基因全长为1872个碱基,单一的开放阅读框架阅读框架编码623个氨基酸的多肽。将测得的序列与澳大利亚六个分离株进行比较,发现我国分离株与渊大利亚分离株间同源性为91%,低于澳大利亚各分 相似文献
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QU Su-jie SHI Kai-chuang SU Yan-qiong HU Jie MO Sheng-lan ZHANG Bu-xian LI Jun ZOU Lian-bin 《中国畜牧兽医》2015,42(12):3119-3125
To investigate genetic variation of avian infectious bronchitis virus (IBV) in Guangxi province,one strain of IBV was isolated from chicken.Two pairs of primers for amplifying the N and M genes of IBV were designed according to the sequences in GenBank.The N and M genes of the strain were amplified by RT-PCR,and they were proved to be the N and M genes of IBV by cloning,sequencing and compared with reference IBV strains published in GenBank.The results showed that the N gene from the IBV isolate consisted of 1 230 bp,coding 409 amino acids.The M gene from the IBV isolate consisted of 678 bp,coding 225 amino acids.The sequence analysis of N gene showed that it shared 87.2% to 93.3% nucleotide homologies and 90.0% to 94.4% deduced amino acid sequence homologies with IBV strains from GenBank.The M gene sequence analysis showed that it shared 83.6% to 91.0% nucleotide homologies and 82.7% to 92.9% deduced amino acid sequence homologies.The phylogenetic tree analysis showed that it was closely related to BJ and LX4 strains,and were clustered into one group;But with the distant relatives from other strains of IBV.These results suggested that the isolate was a new variant of IBV. 相似文献
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为了解狂犬病病毒(RV)的变异情况,本研究对广西不同地区的22个RV分离株的L基因3'端片段进行克隆和测序,与国内外发表的RV街毒、固定毒株及类RV株相应部分的多态性进行了比较分析.结果表明.所测定的22个广西RV野毒分离株属于基因I型,可分为3个群即I群、Ⅱ群和Ⅲ群.其中13株属于I群,其核苷酸同源性为96.9%~100.0%,氨基酸同源性为98.2%~100.0%;8株属于Ⅱ群,株核苷酸同源性为96.5%~99.7%.氨基酸同源性为97.8%~100.0%.仅1株属于Ⅲ群.22个RV分离株与RV固定毒株核苷酸和氨基酸的同源性分别为79.5%~86.9%和85.8%~96.5%,与类RV核苷酸和氨基酸的同源性分别为65.7%~70.3%和70.4%~76.5%. 相似文献
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Nara Pereira EM Iwata H Inoue T 《The Journal of veterinary medical science / the Japanese Society of Veterinary Science》2000,62(3):317-321
The complete nucleotide sequence of cDNA clones representing the L2 dsRNA from Japan isolate of epizootic hemorrhagic disease serotype 2 (EHDV-2JPN) was determined. The EHDV-2JPN L2 gene is 3002 base pairs long with a single open reading frame of 2949 bp which predicts a polypeptide of 982 amino acid residues. Comparison of VP2 sequence between Japan and North American Isolates of EHDV-2 showed a 72% homology in spite of the same serotype, although those among the North American isolates showed a high genetic identity (>97%). 相似文献
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QU Su-jie ZOU Lian-bin HU Jie SU Yan-qiong MO Sheng-lan SHI Kai-chuang YIN Yan-wen LI Jun ZHANG Bu-xian 《中国畜牧兽医》2016,43(1):45-49
To investigate genetic variation of Marek's disease virus(MDV) in Guangxi province, three isolates of MDV were isolated from infected chicken.One pair of primers for amplifying Meq gene of MDV was designed according to nucleotide sequence in GenBank, Meq gene of the isolates were amplified by PCR, and then cloned, sequenced and compared with reference MDV strains published in GenBank.The results showed that Meq gene from all of the MDV isolates consisted of 1020 bp, coding for 339 amino acids.Compared with reference strains published in GenBank, the sequences of Meq gene in different isolates were relatively conserved and the homologies of nucleotide and amino acid sequence of the isolates were 83.8% to 99.9% and 88.4% to 99.6%, respectively.The proline-rich repeats of Meq gene of the MDV isolates had site mutations, and it was related to MDV's virulence.The isolate were nearly related to YL and GXY2, and far away from RB1B, GA, Md5, 648A and the immune strain phylogenetically.The study would provide research materials for the prevalence, genetic variation, protection and control of MDV in China. 相似文献
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为研究鸡马立克氏病病毒(MDV)广西流行株的遗传变异情况,本研究从广西发病鸡中分离鉴定了3株MDV。参照GenBank中MDV的核苷酸序列设计1对引物,利用PCR技术对分离毒株的Meq基因进行了克隆、序列测定,并与GenBank中发表的国内外参考毒株进行比对分析。结果显示, Meq基因序列全长为1020 bp,编码一条由339个氨基酸组成的多肽,分离株与国内外MDV参考毒株相比,不同MDV株的Meq基因序列相对较保守,它们之间核苷酸同源性为83.8%~99.9%,氨基酸同源性为88.4%~99.6%。3株MDV分离株Meq基因在相关报道中提到的与毒力相关的脯氨酸重复区存在点突变。3株分离株与国内参考株YL、GXY2关系较近,与参考株RB1B、GA、Md5、648A及疫苗株亲缘关系较远。该研究为中国MDV的流行、遗传变异及防控研究提供了材料。 相似文献
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为研究新疆地区捕食线虫性真菌的生物活性,本实验采用玉米粉琼脂培养基(CMA)培养分离自新疆不同地区的捕食线虫性真菌,通过对分离株纯培养物的形态学观察和18S rDNA基因序列分析,鉴定4株少孢节丛孢菌,分别命名为XA3、XA6、XD1和XD4。18S rDNA基因遗传进化分析表明,XA3、XA6、XD1和XD4新疆分离株之间同源性较高,与GenBank登录的少孢节丛孢菌CBS289.82株同源性最高,分别为99.6%、99.5%、99.1%和98.9%,与形态学鉴定结果一致。捕食线虫活性测定试验表明,4个分离株在CMA中的捕食率为92.8%~97.6%;体外对绵羊粪便中线虫幼虫的捕食率为90.7%~95.4%,均具有很强的捕食活性。本研究为研究绵羊消化道线虫生物防控制剂奠定基础。 相似文献
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QU Su-jie SHI Kai-chuang ZOU Lian-bin HU Jie MO Sheng-lan YIN Yan-wen ZHANG Bu-xian LI Jun LIANG Yuan 《中国畜牧兽医》2016,43(2):377-382
According to the M gene nucleotide sequence of avian infectious bronchitis virus (IBV) published in GenBank,one pair of primers were designed,the M gene fragments of IBV isolated from Guangxi province were amplified by PCR.Then the amplified fragments were cloned into pMD18-T vector and the positive recombinant plasmids were sequenced.The results showed that M gene from all of the IBV isolates consisted of 678 bp,coding for 225 amino acids.Two glycosylated sites were located nearby the N-terminal,three transmembrane domains were located in the 23 to 98 peptide region.Variations within the hydrophilicity region were easier than that in the hydrophobicity region.Compared with that of other published IBV strains,the homologies of nucleotide and amino acid sequences of the isolates were 83.6% to 92.5% and 82.7% to 95.1%,respectively.The phylogenetic tree analysis showed that it was closely related to SAIB20 and LX4,and clustered into one group;But it belonged to different branches with other reference strains,and had a distant relationship.These results suggested that the isolate was a new variant of IBV. 相似文献
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参照GenBank中鸡传染性支气管炎病毒(IBV)的核苷酸序列设计1对引物,利用 PCR 扩增IBV广西株的M基因片段,将其克隆到pMD18-T载体中.序列分析结果表明,M基因全长为678 bp,编码225个氨基酸,近N端含有2个潜在的N-糖基化位点,3个跨膜区位于23—98肽段区,亲水区较疏水区更易变异.IBV广西株与国内外IBV参考毒株相比,核苷酸序列同源性为83.6%~92.5%,氨基酸序列同源性为82.7%~95.1%.系统进化分析结果显示IBV广西株与SAIB20和LX4两参考株位于同一个分支上,它们的亲缘关系较近,而与其他参考株属于不同的分支,亲缘关系较远.结果表明IBV广西株是1株新的IBV变异株. 相似文献