重组定点突变巴曲酶酶学性质研究

目的对重组定点突变巴曲酶的酶学性质进行研究,为开发成临床用药奠定基础。方法测定不同的温度、pH缓冲液和金属离子等条件对重组定点突变巴曲酶活性的影响。结果重组定点突变巴曲酶的最适pH值在6．5～7．5之间。该酶在50℃以下活力保持90％以上,但当温度超过60℃时,该酶已完全失活。Ca^2＋和Na^＋离子对酶的稳定性无明显影响,而Mg^2＋、K^＋、Mn^2＋离子则表现为激活作用,Zn^2、＋Cu^2＋、Fe^2＋、Co^＋离子则表现为明显的抑制作用。结论重组定点突变巴曲酶在中性条件下比较稳定,它不耐高温,金属离子对其活性有一定的影响。     

重组定点突变巴曲酶质量标准研究

目的 建立重组定点突变巴曲酶的质控方法和质量标准.方法 生物学活性测定采用血浆凝集活性测定法;通过胰蛋白酶消化和RP-HPLC法分析该蛋白还原型肽图;其余检测项目均按<中华人民共和国药典>2010年版(三部)相关规定进行.结果 用建立的方法对三批重组定点突变巴曲酶原液和成品进行检定,各项指标均符合2010版<中华人民共和国药典>和相应指导原则的要求.三批原液比活性均≥2000 kU/mg.肽图三批次之间一致,原液的蛋白含量、纯度、分子质量、等电点、N末端氨基酸序列等指标均符合规定.结论 建立的质控方法可有效地控制重组定点突变巴曲酶产品质量,并可用于定点突变巴曲酶原液及成品的常规检定.     

地高辛标记DNA探针杂交法检测Vero细胞DNA残留量的适用性验证及应用

目的对地高辛标记DNA探针杂交法检测人用狂犬病疫苗(Vero细胞)DNA残留量进行适用性验证及应用。方法对地高辛标记DNA探针杂交法检测人用狂犬病疫苗(Vero细胞)DNA残留量进行特异性、灵敏度及稳定性验证,并应用该方法检测3批人用狂犬病疫苗(Vero细胞)的DNA残留量。结果地高辛标记探针的标记效率为0.1 pg。验证结果显示探针与非同源DNA无杂交;最低检测限度为1 pg;探针在-20℃放置7个月后,检测灵敏度仍可达到1 pg;3批人用狂犬病疫苗(Vero细胞)中残留DNA含量均符合《中国药典》规定质量控制标准。结论地高辛标记DNA探针杂交法特异性、灵敏度好,结果稳定,适用于人用狂犬病疫苗(Vero细胞)中Vero细胞DNA残留量的检测及疫苗生产过程和其成品的质量控制,对其他以Vero细胞为基质的病毒性疫苗质量控制具有借鉴意义。     

地高辛标记探针检测重组人干扰素β_(1b)中DNA残留量

为检测注射用重组人干扰素β1b半成品中外源性DNA残留量,以重组人干扰素β1b工程菌基因组DNA为模板,用地高辛标记探针,并以此探针进行点杂交。结果证明,该方法检测灵敏度较好,特异性较强,操作较安全简便,可用于重组人干扰素β1b制备过程中的质量监控及半成品的检定。     

地高辛标记探针检测生物制品中残余DNA含量

用地高辛标记探针检测由传代细胞系生产的人用精制狂犬病疫苗,重组（CHO细胞）乙肝疫苗,出血热疫苗及痢疾多糖结合疫苗原液中残余DNA含量。结果表明,该方法特异性强,灵敏度高,可用于上述生物制品中残余DNA含量的检测。     

定点突变巴曲酶在毕赤酵母中的克隆与表达

目的 为避免毕赤酵母分泌的Kex2蛋白酶对发酵液中所表达的巴曲酶的降解.利用重叠PCR方法对巴曲酶基因进行定点突变,将巴曲酶基因第45位的Arg突变为Lys.方法 将突变后的基因克隆到酵母分泌型表达载体pPICZαA中,将重组载体酶切线性化后经电转化转入巴斯德毕赤酵母细胞,筛选鉴定转化子,经摇瓶发酵甲醇诱导,酵母菌分泌表达有凝血活性的定点突变巴曲酶,经SDS-PAG电泳、免疫印迹确定其分子量为32 kD.结果发酵罐的表达量达到52 KU/ml发酵液,较重组天然巴曲酶的表达量提高了73.3%.结论 定点突变巴曲酶的表达量比重组天然巴曲酶的表达量有显著提高,表达的突变巴曲酶同样具有凝血活性.     

重组巴曲酶在毕赤酵母中的高效表达

以毕赤酵母为表达系统,建立生产重组巴曲酶的技术工艺路线。通过递归式PCR的方法,人工合成了巴曲酶基因,将其插入pPIC9表达质粒中,转化至毕赤酵母GS115(his4),筛选出的表达株经甲醇诱导,表达了重组巴曲酶,并得以纯化。从每升发酵液中可纯化得到10mg重组巴曲酶,其比活为238NIHunits/mg,分子量为30.55kD。重组巴曲酶在体外可使纤维蛋白凝固,在体内缩短小鼠出血时间。为开发重组的蛇毒类凝血酶止血剂打下了基础。     

地高辛标记探针检测Vero细胞狂犬病疫苗残余Vero细胞DNA含量

地高辛标记Vero细胞DNA,并制备成DNA探针,以此探针进行点杂交,确定探针的工作浓度,特异性及灵敏度,并用此法监测Vero细胞狂犬病疫苗浓缩原液纯化工艺的Vero细胞DNA去除率,测定精制Vero细胞狂犬病疫苗成品中残余Vero细胞DNA含量,结果明显,该法特异性强,重复性好,快速简便,灵敏度高,检测值可达5pg/剂量,可用于精制ero细胞狂犬病疫苗纯化工艺的质量控制和半成品检定。     

地高辛探针检测重组肝靶向干扰素宿主DNA残留量的研究

目的:建立检测重组肝靶向干扰素宿主DNA残留量的方法,根据此法检测3批重组肝靶向干扰素每人份剂量宿主DNA残留量。方法:以重组肝靶向干扰素工程菌基因组DNA为模板,并制备探针,用此标记探针对3批重组产品进行DNA残留量检测。结果:3批次重组肝靶向干扰素原液每人份剂量宿主DNA残留量均小于10 ng。结论:地高辛标记探针斑点杂交检测DNA残留量具有特异性强,灵敏度高,重现性好,操作简单,能快速高效检定重组肝靶向干扰素原液并对其制备过程进行质量监控。     

利用Pyrobest DNA聚合酶一步法进行大片段基因的定点突变

目的:介绍一种简单、快速、高效和经济的进行大片段基因定点突变的方法。方法:小量抽提含有NM23H1-EGFP融合基因的逆转录病毒真核表达质粒pLXSN-NM23H1-EGFP,体外合成突变引物对,利用高保真Pyrobest DNA聚合酶对质粒DNA进行PCR突变反应,然后用DpnⅠ限制性内切酶消化PCR产物以去除模板DNA,取适量消化产物转化大肠杆菌XL1-Blue,随机挑选克隆进行测序筛选、鉴定所需突变株。结果:在NM23H1-EGFP基因中引入了S44A、P96S、H118F、S120G、P96S-S120G等5个替换突变位点及9bp处的插入突变。结论:该方法简单、快速、高效、经济,不须纯化中间产物,不须亚克隆,突变效率几乎为100%,是一种值得推广应用的方法。     

Enhanced photoelectrochemical method for linear DNA hybridization detection using Au-nanopaticle labeled DNA as probe onto titanium dioxide electrode

A photoelectrochemical method was proposed to detect DNA hybridization using Au nanoparticle modified DNA as one probe on TiO2 substrate, in which the TiO2 substrate was used not only as DNA anchors but also as the signal transducers. Hybridization between the probe and the target DNA oligonucleotides was confirmed by the decreased photocurrent of the TiO2 electrode. Compared with non-label probe, Au nanoparticles enhanced the photocurrent shifts after the hybridization. The photocurrent decreased with increasing the concentration of target DNA, indicating that this method could be used for quantitative measurements, and the discrimination of the complementary from mismatched DNA. Furthermore, the hybridization binding constant was obtained and photocurrent generation mechanism was discussed. The major advantages of this photochemical method are speed, simplicity and excellent specificity. This method provides a platform for studying a wide variety of biological processes using photoelectrochemical method.     

A site-targeted recombinant nuclease probe of DNA structure

A genetically engineered lac repressor/T7 endonuclease hybrid protein shows repressor-like binding toward restriction fragments carrying the lac operator. In addition, fragments carrying the operator near a particular pBR322 sequence are cleaved into specific products. Cleavage occurs at precise positions within that sequence, is independent of the orientation of the operator, is inhibited by isopropyl-1-thio-beta-D-galactopyranoside, and is observed when the target is separated from the operator by at least as few as 150 and as many as 240 base pairs. This evidence indicates that the hybrid protein is a site-directed nuclease that requires the following two structural elements for activity: the lac operator and a target. Repressor-like binding directs the enzyme to the operator and nearby single-stranded DNA targets. The discovery of an unusual target in a well-studied DNA sequence is evidence of the power of this approach for probing unusual structures in non-supercoiled duplex DNA.     

光敏生物素和DIG标记Orf病毒DNA探针的研究

目的：是用于Orf病毒病的诊断和相应重组菌的检测,将HCE DNAHindⅢ/A,B片断及重组质粒pGRL-4A中消化的A片断用光敏生物素和地高辛进行标记,对不同病毒分离株DNA进行检测,并对不同重组质粒进行了Dot-blotting和Southem-blotting检测。结果：用光敏生物素标记的探针最低可检出12pg的DNA,地高辛标记的探针最低可检出0.1pg的DNA,且有极强的特异性。     

Quantitation of the residual DNA from rice-derived recombinant human serum albumin

Residual DNA in recombinant protein pharmaceuticals can potentially cause safety issues in clinical applications; thus, maximum residual limit has been established by drug safety authorities. Assays for residual DNA in Escherichia coli, yeast, and Chinese hamster ovary (CHO) cell expression systems have been established, but no rice residual DNA assay for rice expression systems has been designed. To develop an assay for the quantification of residual DNA that is produced from rice seed, we established a sensitive assay using quantitative real-time polymerase chain reaction (qPCR) based on the 5S ribosomal RNA (rRNA) genes. We found that a 40-cycle qPCR exhibited a linear response when the template concentration was in the range of 2 × 10⁴ to 0.2 pg of DNA per reaction in TaqMan and SYBR Green I assays. The amplification efficiency was 103 to 104%, and the amount of residual DNA from recombinant human serum albumin from Oryza sativa (OsrHSA) was less than 3.8 ng per dosage, which was lower than that recommended by the World Health Organization (WHO). Our results indicate that the current purification protocol could efficiently remove residual DNA during manufacturing and processing. Furthermore, this protocol could be viable in other cereal crop endosperm expression systems for developing a residual DNA quantitation assay using the highly conserved 5S rRNA gene of the crops.     

DNA fingerprinting in cattle using the probe pV47

The multilocus probe pV47 detected an average of nine bands in cattle between 23 kb and 4 kb. Band sharing was estimated for three groups of unrelated animals. The first group comprised 20 individuals of 12 different breeds, the second group 10 individuals of the Swiss Simmental population and the third group 11 individuals of the Swiss Brown Swiss population. The band sharing probabilities were 33%, 42% and 58% respectively. The DNA fingerprints of 38 offspring with a total of 277 bands revealed no bands that could not be traced to the parents.