Expression of a recombinant crustacean hyperglycemic hormone of the kuruma prawn Penaeus japonicus in methylotrophic yeast Pichia pastoris

ABSTRACT:   Until now, six crustacean hyperglycemic hormones (CHH) designated Pej-SGP-I, -II, -III, -V, -VI and -VII have been characterized in the kuruma prawn Penaeus japonicus . All CHH consist of 72 amino acid residues and have an amidated carboxyl (C)-terminus. In the present study, we expressed Pej-SGP-III in methylotrophic yeast Pichia pastoris in order to obtain a large quantity of recombinant CHH possessing biological activity. A cDNA encoding Pej-SGP-III that had been previously cloned was processed by polymerase chain reaction (PCR) and the resulting product was ligated into an expression vector. Pichia pastoris was transformed with this vector after which a recombinant Pej-SGP-III was expressed having an additional amino acid residue (glycine) at the C-terminus (rPej-SGP-III-Gly), a form considered to be a putative precursor of this hormone. rPej-SGP-III-Gly secreted into the culture medium was purified by reversed-phase HPLC, and amidated using a peptidylglycine alpha-amidating enzyme. The amidated rPej-SGP-III (rPej-SGP-III) showed hyperglycemic activity in in vivo bioassay almost comparable to that of the natural Pej-SGP-III. rPej-SGP-III thus obtained will be a useful tool not only for its physiological study but also for the determination of its 3-D structure.     

利用反向遗传技术拯救H9N2重组病毒

为研制高效特异的H9N2亚型AI疫苗,选取我国具有代表性的毒株A/chicken/Shanghai/10/01(H9N2)(简称SH10),以12质粒系统为基础,利用反向遗传操作技术构建了1株表面基因由SH10提供、内部基因由12质粒系统提供的重组病毒SH/PR8,为新型疫苗的研制提供了新的毒株。     

Molecular cloning,purification and immunogenicity of recombinant Brucella abortus 544 malate dehydrogenase protein

The Brucella mdh gene was successfully cloned and expressed in E. coli. The purified recombinant malate dehydrogenase protein (rMDH) was reactive to Brucella-positive bovine serum in the early stage, but not reactive in the middle or late stage, and was reactive to Brucella-positive mouse serum in the late stage, but not in the early or middle stage of infection. In addition, rMDH did not react with Brucella-negative bovine or mouse sera. These results suggest that rMDH has the potential for use as a specific antigen in serological diagnosis for early detection of bovine brucellosis.     

表达H3N2亚型猪流感病毒HA基因重组伪狂犬病病毒的构建

将SV40启动子控制下的LacZ基因表达盒和CMV启动子控制下的H3N2亚型猪流感病毒（SIV H3N2）的HA基因插入到伪狂犬病病毒（PRV）通用转移载体pBdTK-Uni中，获得转移载体pLTK-HA。将该载体与PRV Bartha-K61株基因组DNA通过脂质体法共转染Vero细胞，经过10代蓝斑筛选、纯化和PCR鉴定获得了一株插入SIV HA基因的重组伪狂犬病病毒，命名为rPRV-HA。Western blotting和间接免疫荧光试验证实HA基因在重组病毒感染的细胞中获得了表达。用不同的细胞（PK-15、IBRS-2、Vero和鸡胚成纤维细胞）对该重组病毒与亲本病毒的增殖滴度和致细胞病变进行比较，未见显著差异，对第30代重组病毒的HA基因进行序列分析，表明该重组病毒遗传性状稳定。     

亚洲1型口蹄疫病毒L蛋白缺失株的构建及其生物学定性

为确定口蹄疫病毒(FMDV)L蛋白缺失对其生物学特性的影响,本研究在已建立的Asia1型FMDV反向遗传操作平台基础上,利用融合PCR方法缺失L蛋白基因编码区,构建了缺失L蛋白的重组Asia1型FMDV(rFMDV-ΔL)。拯救病毒的一步生长曲线结果表明,rFMDV-ΔL与亲本病毒相比在BHK-21细胞中的复制水平下降10倍,乳鼠毒力试验表明rFMDV-ΔL的毒力比亲本毒株下降6倍。另外,rFMDV-ΔL在BHK-21细胞上产生病变的速度明显变慢,形成蚀斑的时间延长,致乳鼠死亡所需时间也比亲本毒株明显延长。本研究是关于亚洲1型FMDVL蛋白结构与功能研究的首次报道,为亚洲1型FMDVL蛋白结构与功能的研究奠定了基础。     

自身启动子控制的卡那霉素抗性基因在哺乳动物细胞中表达的检测

为了研究卡那霉素抗性(KanR)基因能否在哺乳动物细胞中表达以及用含相同抗性基因重组质粒防治奶牛乳腺炎的安全性,用PCR从重组质粒p215C3LYZ中扩增得KanR基因,将其克隆入原核表达载体pQE-31,用含卡那霉素(Kan)琼脂平板筛选得KanR重组菌,经IPTG诱导成功表达了预期大小的Kan抗性融合蛋白;用纯化的重组蛋白免疫小鼠,获得了Kan抗性蛋白抗血清,经Western blotting证明免疫血清特异性良好;分别用重组质粒pQE-Kan和p215C3LYZ转染COS-1细胞,在不含抗生素培养液中培养后分别收集细胞上清和细胞裂解物;将转染细胞上清分为添加和不加Kan组,接种Kan敏感菌DH5α大肠杆菌,培养物的OD600检测结果显示,添加组的指示菌生长被抑制,转染细胞上清中无Kan抗性蛋白表达;以Kan抗性蛋白免疫血清进行的Western blotting结果显示,转染细胞内无Kan抗性蛋白表达;将p215C3LYZ注射奶牛乳腺,用脱脂和浓缩奶样进行Western blotting检测,结果显示试验牛乳中也无Kan抗性蛋白表达。这些试验结果提示,来源于原核大肠杆菌的KanR基因启动子在动物细胞中无转录活性,乳腺注射含KanR基因的重组质粒不会表达对奶牛和人体有害的Kan抗性蛋白。     

表达新城疫病毒F基因重组鸡痘病毒的筛选

将转移载体P11SF和PN11SF分别与282E4株鸡痘病毒（282E4 strain fowlpox virus，282E4FPV）和大空斑株鸡疽病毒（large plaque strain fowlpox virus，LP FPV）共转染鸡胚成纤维细胞，通过蓝斑筛选，得到4株重组鸡痘病毒rFPV282E4-SFA、rFPVLP，-SFA、rFPV282E4-SFB和rFPVLP-SFB，通过PCR和间接免疫荧光鉴定均为阳性，另外将各重组病毒分别传20代，测其遗传稳定性，结果显示均具有良好的稳定性。对SPF鸡进行免疫效力试验，攻毒后均100％保护，而对于商品鸡，保护率分别为64％、60％、52％和88％。     

Gene cloning of porcine adiponectin gene from adipose tissue and construction of its eukaryotic expression vector

To clone adiponectin (ADPN) gene from Shaziling porcine adipocyte and construct its eukaryotic expression vector, total RNA was extracted from subcutaneous fatty tissue. One pair of specific primers was designed by Primer 5.0 software according to the sequence of ADPN gene of porcine available in GenBank. The ADPN gene was amplified by PCR from cDNA and cloned into pMD18‐T vector to construct recombinant clonal vector pMD‐ADPN, sequenced and analysed. A recombinant expression plasmid pPICZaA‐ADPN was constructed by subcloning the cloned ADPN gene into the linearized pPICZaA vector. Then, the plasmid pPICZaA‐ADPN was expressed in Pichia pastoris (GS115) by electrotransformation. Western blot and Bradford analysis were used to determine the target protein induced by methanol. Results showed that the genome size of ADPN was 732 bp and encoded 244 amino acid, the nucleotide sequence of ADPN shared 100% identity with that of porcine available in GenBank. Western blot and Bradford analysis showed that the recombinant ADPN was expressed in GS115 correctly and has certain immune activity. The expression level of ADPN was 28.5 μg/ml. In conclusion, the recombinant ADPN could express in eukaryotic expression vector pPICZaA‐ADPN constructed in this study effectively.     

猪细小病毒BQ-C毒株VP2基因的鉴定及表达

本研究从临床发病猪采集病料,以PK15传代细胞进行病毒分离,通过PCR、血液凝集试验(HA)和电镜鉴定为1株猪细小病毒(porcine parvovirus,PPV),命名为BQ-C。对分离的毒株进行测序,结果显示该毒株与GenBank登录的PPV BQ株同源性为100%。为获得该毒株结构蛋白VP2基因的表达产物,将VP2基因片段插入到原核表达载体pET-30a(+),得到表达重组质粒。经双酶切和测序鉴定,将重组质粒转化大肠杆菌BL21(DE3)中进行表达。SDS-PAGE结果表明,获得的重组蛋白分子质量约为71.5 ku,与预期大小相符。Western blotting结果显示获得的重组蛋白能与PPV阳性血清特异性结合,表明重组蛋白具有良好的反应原性。结果表明,本研究成功分离了1株PPV BQ-C株,且表达的VP2重组蛋白可用于PPV血清学诊断和疫苗的研发。     

麋鹿重组朊蛋白单克隆抗体的制备及初步鉴定

为研制鹿慢性消耗性疾病(chronic wasting disease,CWD)单克隆抗体,本研究以原核表达后经纯化的麋鹿重组成熟朊蛋白(PrP^c)为免疫原免疫PrP^c基因敲除小鼠(PrP^c-null mice)。两次加强免疫后,利用淋巴细胞杂交瘤技术,取脾细胞与SP2/0骨髓瘤细胞进行细胞融合,间接ELISA方法筛选阳性杂交瘤细胞,采用3次有限稀释法实现杂交瘤细胞的亚克隆,筛选出5株能稳定分泌针对麋鹿重组成熟朊蛋白特异性单克隆杭体(McAbs)的杂交瘤细胞株5A5、3B2、6D12、5E3、1F5,其腹水ELISA效价均达到1∶10000以上。经鉴定,5株单抗均为IgG抗体,5A5、6D12、5E3株为IgG1亚类,3B2、1F5株为IgG2a亚类。Western blotting鉴定结果表明,获得的McAbs均能特异性识别麋鹿重组成熟朊蛋白和健康麋鹿脑组织匀浆中的PrP^c。本研究制备了CWD腹水McAbs,同时也为CWD的研究及其诊断方法的建立奠定了基础。