摘要
猪繁殖和呼吸综合征病毒(PRRSV)的基质膜(M)蛋白和核衣壳(N)蛋白是2种重要的结构蛋白。本试验根据PRRSV美洲毒株的基因序列,设计了能够扩增M和N蛋白基因的1对引物,并在2个引物的两端分别加入EcoRI和BamHI酶切位点,经RT-PCR技术获得了一约950bp的目的基因片段,并将此基因克隆于PBV220载体,构建了MN蛋白基因重组质粒PBVMN,进一步由重组质粒回收MN基因片段亚克隆于pSK+(pBluescriptSK+)测序载体,构建了重组质粒PBSMN,经部分序列分析鉴定,重组质粒含MN蛋白基因。此基因的克隆为进一步研究该病毒MN蛋白免疫学特性及其分子基础和基因诊断技术奠定了基础。
Matrix membrane (M) protein and nucleocapsid (N) protein of PRRSV are two important structural proteins. Primers for RT PCR were designed on the basis of VR2385 isolate sequence of US PRRSV which amplified the entire protein coding regions of the M and N genes. Unique restriction sites (Eco RI and Bam HI) at the termini of the PCR products were introduced. A PCR product with the expected size of about 950 bp was obtained from a modified live PRRSV. The PCR product of the M and N genes from PRRSV was then digested with Eco RI and Bam HI, purified and cloned into vector PBV220 and one recombinant PBVMN was constructed. The M and N gene of PBVMN was further subcloned into vector pSK + (pBluescript SK +) and one recombinant PBSMN was obtained. A partial sequence of PBSMN containing the full length of M and N genes was identified with an automated DNA sequencer. The report provides some valuable materials for investigation of M and N protein antigenic properties and molecular characteristics as well as genomic diagnostic technique of PRRSV.
出处
《中国兽医学报》
CAS
CSCD
北大核心
1999年第1期3-6,共4页
Chinese Journal of Veterinary Science
基金
国家自然科学基金
关键词
猪
基因克隆
MN蛋白
PRRSV
病毒
核衣壳
膜蛋白
pig
porcine reproductive and respiratory syndrome virus
gene cloning
MN protein gene
