棉铃虫核多角体病毒iap3基因表达时相分析

目的:原核表达棉铃虫核多角体病毒(Helicoverpa armigera nucleopolyhedrovirus,HearNPV)iap3基因,制备该蛋白的多克隆抗体,并利用该抗体分析iap3基因在病毒感染过程的表达时相,为深入研究提供基础.方法:PCR扩增iap3基因后,克隆至pET28b,转化到大肠杆菌BL21 (DE3)中诱导表达,利用亲合层析进行蛋白纯化,将纯化融合蛋白免疫大鼠制备抗血清,利用抗血清Western blot检测IAP3在病毒感染过程的表达时相.结果:成功在原核细胞中表达iap3基因,并获得纯化的融合His - tag的IAP3蛋白,制备了该蛋白的多克隆抗体.发现iap3基因最早在感染后24h表达,到72h到达表达高峰.结论:获得了IAP3多克隆抗体,iaP3基因是一个晚期表达基因.     

斜纹夜蛾核型多角体病毒ⅡORF146基因的克隆、表达与启动子活性分析

【目的】研究斜纹夜蛾核型多角体病毒II ORF146基因的结构与功能。【方法】根据SpltMNPV IIORF146基因序列设计引物,经PCR扩增克隆ORF146基因。在生物信息学分析基础上进行启动子活性分析和转录时相分析。构建ORF146片段的原核表达载体,表达并纯化融合蛋白后制备多克隆抗体。【结果】核苷酸序列分析表明,读码框含1383 bp,编码460个氨基酸的蛋白质,推定分子量为50.4 kDa。启动子活性分析和转录时相分析都表明该基因是个早、晚期都表达的基因,在病毒感染8 h和18 h有两个转录峰,24 h以后转录水平略有下降,但趋于稳定。pET-28a-ORF13原核表达的融合蛋白经纯化后制备的多克隆抗体特异性高,效价可达1∶3200以上。【结论】SpltMNPV II ORF146基因是一个早期和晚期都表达的病毒组成型结构蛋白基因。推测ORF146基因可能与SpltMNPV II病毒感染宿主细胞后病毒DNA复制有关。制备的多克隆抗体可用于深入研究该蛋白的生物学特性与功能。     

家蚕核型多角体病毒orf25基因在病毒感染过程中 编码一个30kDa的晚期蛋白

首次对家蚕核型多角体orf25基因进行了描述.扩增Bm25基因,亚克隆到原核表达载体pGEX-4T-2,在大肠杆菌BL21(DE3)中表达含有GST标签的融合蛋白.IPTG诱导后高效表达GST-Bm25融合蛋白.纯化的融合蛋白免疫新西兰大白兔制备多克隆抗体.利用制备的抗GST-Bm25融合蛋白的多克隆抗体进行表达时相分析显示:24 h p.i.检测到30 kDa的蛋白条带.RT-PCR方法,在18-72 h p.i 检测到Bm25基因的转录本.结论:以上数据表明Bm25基因编码一晚期表达的30kDa蛋白.     

杆状病毒ac68基因的克隆、表达与抗体制备

目的：对苜蓿丫纹夜蛾核多角体病毒（Autographa califorica multicapsid nucleopoly hedrovirus,AcMNPV）开放阅读框68（open reading frame,ORF68,ac68）进行原核表达,制备该蛋白的多克隆抗体,为深入研究其功能提供基础。方法：将ac68基因克隆至原核表达载体pET28a上,在大肠杆菌BL21（DE3）中表达Ac68蛋白,通过His抗体检测进一步验证所表达的蛋白为带有组氨酸的融合蛋白。以纯化的Ac68蛋白作为抗原,免疫昆明小鼠制备多克隆抗体。结果：实现了ac68基因的原核表达,获得了该蛋白的多克隆抗体并在AcMNPV感染的Sf-9细胞中检测到一条大小为25kD左右的特异杂交带。结论：获得的抗体可用于Ac68蛋白功能的进一步研究。     

人类博卡病毒(HBoV)非结构蛋白NS1基因的克隆、原核表达及多克隆抗体的制备

目的:克隆、表达、纯化人类博卡病毒(HBoV)非结构蛋白NS1,制备抗NS1多克隆抗体。方法:利用PCR扩增HBoV非结构蛋白NS1基因,将其克隆至pMAL-c2X表达载体上,重组质粒转化大肠杆菌DH10B,IPTG诱导表达。表达的融合蛋白经Amylose Resin亲和层析柱纯化后,免疫新西兰大白兔制备多克隆抗体。用间接ELISA法检测抗体效价。结果:原核表达融合蛋白MBP-NS1,并获得了其多克隆抗体,抗体效价达到1∶32000。结论:在原核表达系统中表达、纯化了融合蛋白,制备抗NS1多克隆抗体,为进一步研究该病毒非结构蛋白基因的转录和翻译机制提供可靠的工具。     

跨膜逆向转运蛋白NHXFS1多克隆抗体的制备及应用

NHXFS1基因是通过DNA家族改组（DNA family shuffling）技术,以拟南芥、水稻和菊花的液泡膜Na＋/H＋逆向转运蛋白基因（NHX1）为亲本获得的活性显著增强的新基因。为制备该蛋白的多克隆抗体,对该蛋白进行跨膜结构分析,选取跨膜蛋白的C末端为靶标,并将其克隆到原核表达载体pET32a中,成功构建了原核融合蛋白pET32a-NHXFS1-抗原表达载体,转化大肠杆菌BL21（DE3）并诱导表达。通过镍柱亲和层析纯化该融合表达蛋白,获得了纯度约为80%的纯化蛋白,用于免疫新西兰大白兔制备多克隆抗体。ELISA实验表明,该抗体的效价达到1：128 000,提取表达NHXFS1蛋白的酵母液泡经该多克隆抗体Western blot检测,证明该抗体具有较好的NHXFS1蛋白特异性。NHXFS1多克隆抗体的制备为进一步认识NHXFS1新蛋白结构与功能以及植物耐盐分子生物学的研究奠定了基础。     

杆状病毒SpltMNPV ORF124基因截短片段的克隆与表达

目的:克隆并表达斜纹夜蛾核多角体病毒(Spodotura litura mulfieapsid nucleopolyhedrovirus,SpltMNPV)ORF124基因的部分编码序列.方法:用PER方法扩增目的基因序列片段,并将其克隆至原核表达载体pQE-30上,转化到Escherichia.coli M15[pREP-4]中进行诱导表达.结果:构建了pQE-tr124原核表达质粒,含有该质粒的大肠杆菌经IPTG诱导表达了一个与预期理论值相符的约为33kDa的蛋白.以Ni2+-NTA偶连抗体检测证明所表达的蛋白为带有组氨酸的融合蛋白.结论:成功表达了SpltMNPV ORF124的部分编码序列,该融合蛋白的成功表达为进一步深入研究基因的功能奠定了基础.     

C19orf18蛋白的表达与纯化及多克隆抗体制备

旨在得到较高浓度和纯度的C19orf18蛋白,再将得到的目的蛋白用于制备其特异性的多克隆抗体。利用PCR技术扩增出C19orf18基因的胞内段和胞外段,中间用柔性肽连接,再将目的片段克隆到p ET28a(+)与p ET32a(+)载体上,通过诱导表达少量的目的蛋白,筛选出表达量较高的载体,再用筛选得到的表达量较高的载体大量表达目的蛋白,通过镍柱纯化得到较纯的C19orf18蛋白。用得到的蛋白免疫新西兰白兔,得到的抗血清先经过Protein A纯化,再进行抗原亲和纯化得到C19orf18蛋白多克隆抗体。结果显示,载体p ET28a-C19orf18蛋白表达量高于p ET32a-C19orf18,经过镍柱纯化后得到了较高浓度与纯度的目的蛋白,利用得到的目的蛋白作为抗原成功制备了其特异性的多克隆抗体。在原核细胞中成功表达了C19orf18重组蛋白,并得到了其特异性多克隆抗体,所制备的多克隆抗体可应用于ELISA、蛋白免疫印迹实验。     

LPTS抗体的制备和活性检测

LPTS是利用定位候选克隆策略 ,得到的一个新的肝相关候选肿瘤抑制基因 (anovelliver relatedputativetumorsuppressor) ,为了进一步研究其结构与功能 ,利用DNA重组技术 ,将LPTS的cDNA克隆到融合表达载体pET 2 4a中 ,在E .coli中表达 ,以Ni+柱亲和层析 ,获得纯化的 6×His LPTS融合蛋白。以此为抗原免疫新西兰大白兔获得多克隆抗体 ,ELISA法检测其滴度达 2 0 0 0 0以上 ,经亲和层析纯化 ,Western印迹结果表明 ,该纯化抗体可与真核表达的HA LPTS蛋白和内源性的LPTS蛋白特异性结合 ;免疫荧光分析显示SMMC 772 1细胞内源性表达的LPTS蛋白呈点状分布于细胞核内。以上结果表明获得了效价高 ,活性强的针对LPTS蛋白的多克隆抗体 ,可用于对LPTS的结构和功能研究。     

人类心脏和肌肉组织特异表达基因Smyd1的表达与抗体制备

Smydl基因是人类心脏和肌肉特异表达基因．制备该基因的多克隆抗体可以为进一步深入研究Smydl在心脏发育过程中与其他因子相互作用提供检测工具．通过PCR方法扩增smydl基因的编码区片段．并将其克隆至PGEX-4T-1上,转化到大肠杆菌BL21（DE3）中,再通过5052法和IVrG法分别诱导表达GST-Smydl融合蛋白．经比较,5052法诱导的蛋白表达量明显高于IPTG法．采用5052法大量诱导表达,通过割胶回收纯化融合蛋白,免疫新西兰大白兔制备多克隆抗体,Westernblot检测抗体活性．结果表明。实验获得了高质量的多克隆抗体．     

重组C8orf32蛋白的表达、纯化及抗体制备

C8orf32是一种功能未知基因,其mRNA含量在乳腺癌组织中显著高于正常乳腺组织。将其开放式阅读框插入pGEX-6P1原核表达载体T7启动子控制下的GST编码基因下游,构建了C8orf32蛋白表达质粒pGEX-6P-C8。表达质粒转化入大肠杆菌BL21(DE3)菌株,经IPTG诱导,成功表达了GST- C8orf32融合蛋白。经带有GST标签的位点特异性蛋白酶切割除去GST-C8orf32融合蛋白的GST标签,获得了N端带有8个多余氨基酸残基的C8orf32蛋白,蛋白纯度为95%左右。N端氨基酸序列分析表明该蛋白N端氨基酸序列正确,质谱鉴定进一步证明所表达C8orf32蛋白的正确性。用制备的C8orf32蛋白免疫新西兰白兔,获得了能够正确识别C8orf32蛋白的抗血清。该蛋白及其抗体的成功制备,为进一步研究C8orf32蛋白的结构功能和体内分布打下了基础。     

Prokaryotic expression and potential application of the truncated PCV-2 capsid protein

Three pairs of specific primers were designed to amplify the F2-1, F2-2 and XF2-2 truncated sequences of ORF2 which encodes the capsid protein of porcine circovirus type 2 (PCV-2). The F2-1 sequence had most of the NLS region of ORF2, but the F2-2 and XF2-2 genes had the NLS region deleted. Truncated genes were subcloned into pET-32a(+) vectors to construct recombinant fusion expression vectors. The vectors were then transformed into Rosetta(DE3) E. coli and expressed by induction of IPTG. Expressed proteins were detected by western blotting and ELISA. The protein with best immunoreactivity was confirmed and selected, then utilized to inoculate SPF rabbits to prepare polyclonal antibodies. The protein and prepared polyclonal antibody were utilized to detect sera samples against PCV-2 from Shandong province and PCV-2 particles in PK-15 cells. In our study, three recombinant fusion proteins were successfully obtained, and the molecular weights of fusion proteins were 35.9 kDa, 33.6 kDa and 38.6 kDa respectively detected by SDS-PAGE. All of the proteins showed positive reaction with anti-PCV-2 antisera, and His-XF2-2 showed better immunoreactivity than the others. The protein of His-XF2-2 was coated as antigen in ELISA to detect the seroprevalence of PCV-2 in certain districts of Shandong province, the seropositivity rate was 27.7 % (73/264). Specific fluorescence and positive signals for PCV-2 could be detected in PK-15 cells inoculated with PCV-2 with the participation of prepared antibodies against His-XF2-2 in IFA and IPMA. Experimental results indicated that the truncated PCV-2 ORF2 gene containing most of the NLS region was successfully expressed in E. coli, and His-XF2-2 was demonstrated to have better immunoreactivity with anti-PCV-2 antisera than the other two fusion proteins. His-XF2-2 and prepared polyclonal antibodies against it had a satisfactory capability in detecting PCV-2 infection.     

The plant mitochondrial open reading frame orf221 encodes a membrane-bound protein

We have shown that the open reading frame orf221 is an active mitochondrial gene which encodes a novel mitochondrial polypeptide. The orf221 sequence is common to higher plants but absent in animal and fungal mitochondria. A mitochondrial polypeptide with an apparent molecular weight of 21 000 was detected with a polyclonal antibody raised against an ORF221 fusion protein. In organello translation followed by immunoprecipitation with the anti-ORF221 antibody demonstrated that this polypeptide is encoded by the orf221 gene in plant mitochondria. The ORF221 was found to be a mitochondrial membrane protein in normal (N), cms-T, and cms-C cytoplasms of several inbred lines of maize (Zea mays L.) and in other plant species.     

单克隆非特异性抑制因子—β（MNSFβ）在大肠杆菌中的表达、抗体的制备及在小鼠子宫内膜上的组织定位

为了获得足够量的单克隆非特异性抑制因子-β蛋白（monoclonal nonspecific supressor factorβ,MNSFβ）及其抗体用于探讨MNSFβ在着床中的作用机理,本研究构建了表达质粒pBV220/MNSFβ-hCCβ,在大肠杆菌中表达了融合蛋白MNSFβ-hCCβ,用抗hCGβ抗体对表达产物进行鉴定,结果表明融合蛋白MNSFβ-hCGβ得到了正确表达,且分子量和理论值相近,表达产物MNSFβ-hCGβ经初步纯化后用于免疫Balb/C小鼠,制备抗体,同时,我们还构建了表达质粒pGEX-4T-2/MNSFβ,在大肠杆菌中表达了融合蛋白GST-MNSFβ,用融合蛋白GST-MNSFβ对融合前的免疫小鼠回忆刺激并进行检测,制备了抗MNSFβ多克隆抗体和单克隆抗体,应用所制备的多克隆抗体进行免疫组化研究,对MNSFβ在小鼠子宫内膜上进行了组织定位,结果显示,MNSFβ在着床日（受精后第4.5天）小鼠子宫非着床位点的表达和着床位点相比明显提高。     

Characterization of two monoclonal antibodies, 38F10 and 44D11,against the major envelope fusion protein of Helicoverpa armigera nucleopolyhedrovirus

The envelope fusion protein F of baculoviruses is a class I viral fusion protein which play a significant role during virus entry into insect cells. F is initially synthesized as a precursor(F_0) and then cleaved into a disulfide-linked F_1 and F_2 subunits during the process of protein maturation and secretion. To facilitate further investigation into the structure and function of F protein during virus infection, monoclonal antibodies(mAbs) against the F_2 subunit of Helicoverpa armigera nucleopolyhedrovirus(HearNPV)(Ha F) were generated. Two kinds of mAbs were obtained according to their different recognition epitopes: one kind of mAbs, as represented by 38F10,recognizes amino acid(aa) 85 to 123 of F_2 and the other kind, represented by 44D11, recognizes aa148 to 173 of F_2. Western blot and immunofluorescence assay confirmed that both of the mAbs recognized the F protein expressed in HearNPV infected cells, however, only 44D11 could neutralize HearNPV infection. The results further showed that 44D11 may not interact with a receptor binding epitope, rather it was demonstrated to inhibit syncytium formation in cells expressing the Ha F protein. The results imply that the monoclonal antibody 44D11 recognizes a region within HaF_2 that may be involved in the F-mediated membrane fusion process.     

Bacterial expression of an immunologically reactive PCV2 ORF2 fusion protein

The entire coding region of open reading frame 2 (ORF2) of porcine circovirus 2 (PCV2) was linked to the 3'-end of the maltose-binding protein (MBP)-His(8)-tag gene. The fusion protein was expressed as soluble form after induction by isopropylthio-beta-d-galactoside. MBP-His(8)-ORF2 was purified to homogeneity by immobilized metal affinity chromatography based on the interaction of the polyhistidine-tag with metal ions. Expression could represent 1% of the total protein in Escherichia coli, allowing approximately 1 mg of highly purified protein to be obtained per liter of bacterial culture. The fusion protein was recognized in Western blot by anti-PCV2 polyclonal antibody and swine sera with PCV2 infection. In addition, rabbit polyclonal antibody raised against purified MBP-His(8)-ORF2 fusion protein reacted with the ORF2 protein in immunoprecipitation. The availability of this fusion protein should permit a thorough study of prevalence of PCV2 infection in large-scale serological studies of field samples.     

Immunogenicity Analysis of Prokaryotic Expression Products of Kaposi＇s Sarcoma Associated Herpesvirus orf65

To purify the protein encoding the small capsid protein (SCP) of KSHV and analyze its immunogenicity, the carboxyl terminus of orf65 of Kaposi's sarcoma associated-herpesvirus (KSHV) was expressed in a prokaryotic expression system. The expression of recombinant E. coli containing pQE-80L-orf65 was induced by isopropyl-β-D-thiogalactopyranoside (IPTG) and the fusion protein was purified by chromatography. The expressed protein and its purified product were identified by sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) and showed that 9 kDa was the expected size of the purified orf65 protein. The antiserum was produced in rabbit which was immunized by purified orf65 protein. An ELISA assay was established to analyze the immunogenicity of the purified orf65 protein. The ELISA analysis demonstrated that orf65 protein has strong immune activity, and the immune activity of polyclonal antibody against orf65 was more than 4 fold higher than that in the serum of the non-immunized rabbit. These results demonstrate that purified orf65 protein has very strong immunogenicity and can be used in screening KSHV infection in the general population using ELISA.