柯萨奇B3病毒结构和非结构蛋白基因重组质粒的构建及其在体外真核细胞中的

制备ＣＶＢ３结构蛋白和非结构蛋白重组质粒ＤＮＡ疫苗时,采用ＲＴ－ＰＣＲ从ＣＶＢ感染的ＨｅＬａ细胞中扩增ＶＰ１、ＶＰ２、２Ａ和３Ｄ基因,重组入真核表达质粒ｐｃＤＮＡ３中,构建ｐｃＤＮＡ３／ＶＰ２、ｐｃＤＮＡ３／ＶＰ１、ｐｃＤＮＡ３／２Ａ和ｐｃＤＮＡ３／３Ｄ重组质粒,经酶切和测下实扩增的序列并将各重组质粒体外转染真核细胞ＣＯＳ－７,用ＲＴ－ＰＣＲ检测ｍＲＮＡ的转录,用Ｗｅｓｔｅｒｎ－ｂｌｏｔ检测表达产物。结果４种重组质粒酶切出相应大小的目的片段,经测序证实为ＣＶＢ３相应序列,Ｗｅｓｔｅｒｎ－ｂｌｏｔ证实能够在体外真核细胞中表达。本文成功构建ＣＶＢ３结构与非结构蛋白的重组质粒ＤＮＡ疫苗,为进一步研究其免疫效果奠定了基础。     

重组人血小板生成素在大肠杆菌中表达的研究

采用化学法全合成了编码人血小板生成素（ｔｈｒｏｍｂｏｐｏｉｅｔｉｎ,ＴＰＯ）成熟肽Ｎ端１５３氨基酸的基因序列,构建基于该合成基因的表达质粒,结果以谷胱甘肽转硫酶－ＴＰＯ１５３（ＧＳＴ－ＴＰＯ１５３）融合蛋白的方式获得了占全菌蛋白４０％的高效表达．进一步采用ＰＣＲ方法分别对ＴＰＯ合成基因及ＴＰＯｃＤＮＡ的翻译起始区（ＴＩＲ）序列进行定点突变,以降低这一区域的Ｇ－Ｃ含量．将突变序列分别插入到ｐＢＶ２２０表达载体中,重组质粒在转化大肠杆菌ＪＭ１０９后,均获得了表达,其中ＴＩＲ区突变后的合成基因表达产物约占全菌蛋白的１５％．为研究基因下游结构对表达的影响,在不改变氨基酸组成的基础上,构建了ＴＰＯ合成基因与ＴＰＯｃＤＮＡ的杂合序列表达质粒．研究结果表明翻译起始效率是影响ｒｈ－ＴＰＯ在大肠杆菌中表达的重要因素之一,同时基因下游序列的组成对表达水平也会产生影响．     

BRCA1基因结构及其在乳腺癌中的表达

利用ＭＰＣＲ技术从乳腺组织分离到抑癌基因ＢＲＣＡ１的ｃＤＮＡ片段,将此９１４ｂｐ的片段克隆进质粒ｐＵＣ１１８,并经全序列测定证实。序列分析表明,ＢＲＣＡＩｃＤＮＡ编码的肽链ＮＮ２－末端有一锌指结构,抑癌基因ＢＲＣＡＩ的产物可能是ＤＮＡ结合蛋白,ｃＤＮＡ序列存在两个变异位点：一个是第４０９位的Ｃ→Ａ（Ａｓｐ→Ｇｌｕ）：另一个是第８７９位的Ａ→Ｔ（ＭＩａ同义突变）。以该片段为探针,检测６例乳腺癌组织中ＢＲＣＡＩｍＩＭＡ表达,一例表达明显下降,一例没检测到表达的ｍＩＭＡ产物,说明一些乳腺癌组织的ＢＲＣＡ１基因转录水平降低     

牛疱疹病毒Ⅰ型前早期基因BICPO的表达对牛免疫缺陷病毒LTR的反式激活作用

由含有ＢＨＢＶ－１（ＢｏｖｉｎｅＨｅｒｐｅｓＶｉｒｕｓ－１）前早期基因的基因组片段亚克隆ＢＩＣＰＯ（ＢＨＶ－１ＩｎｆｅｃｔｅｄＣｅｌｌＰｒｏｔｅｉｎＯ）的ＤＮＡ序列至表达载体ｐＳＶＫ３,构建质粒ｐＳＶ２．９。将该质粒与ｐＢＬＴＲ－Ｌｕｃ共转染小牛肺细胞,检测转染细胞裂解物的荧光素酶活性,ＢＩＣＰＯ的表达产物可以显著地激活ＢＩＶＬＴＲ启动子控制下的荧光素酶基因的表达。根据ｐＳＶ２．９与含有ＢＩＶＬＴＲ不同区段缺失的质粒ｐＤ－３１９－Ｌｕｃ、ｐＤ－１１５－Ｌｕｃ、ｐＤ－５２－Ｌｕｃ共转染小牛肺细胞的实验结果,推测ＢＩＶＬＴＲ－３１９位上游区的ＤＮＡ序列影响ＢＩＣＰＯ基因产物对ＢＩＶＬＴＲ表达的激活作用。     

人血小板生成素(hTPO)全长 cDNA 克隆及在 CHO 细胞中的表达

以人胎肝ｍＲＮＡ为模板,采用ＲＴ-ＰＣＲ扩增了人ＴＰＯ编码区全长ｃＤＮＡ,全序列测定结果表明与国外报道序列一致;进而构建了ｐｃＤＮＡ３-ＴＰＯ永久表达载体,转染ＣＨＯ细胞后经Ｇ４１８加压筛选、ＴＰＯ表达稳定性等项指标测试,获得了稳定分泌ＴＰＯ的工程细胞株。     

人血小板生成素（hTPO）的cDNA克隆,序列测定及其在COS—7细胞中的表达

本文利用反转录ＰＣＲ技术从人胎肝ｍＲＮＡ中分别扩增出ｈＴＰＯ　Ｎ－端和Ｃ－端两个ｃＤＮＡ片段,然后经酶切分别连接重组到质粒ｐＵＣ１９中进行序列分析,在确证其序列与国外文献报道完全一致的基础上,酶切、回收、连接其Ｎ－端、Ｃ端ｃＤＮＡ,并以此为模板,用ＰＣＲ法扩增出全长ＴＰＯｃＤＮＡ片段,并将其重组到穿梭质粒ｐＳＶＫ３中,在ＣＯＳ－７中进行了瞬时表达并检测出表达产物的活性     

人血小板生成素（hTPO）全长cDNA克隆及其在CHO细胞中的表达

以人胎肝ｍＲＮＡ为模板,采用ＲＴ－ＰＣＲ扩增了人ＴＰＯ编码区全长ｃＤＮＡ,全序列测定结果表明与国外报道序列一致;进而构建了ｐｃＤＮＡ３－ＴＰＯ永久表达载体,转染ＣＨＯ细胞后经Ｇ４１８加压筛选、ＴＰＯ表达稳定性等项指标测试,获得了稳定分泌ＴＰＯ的工程细胞株。     

抗人CD3单抗重,轻链可变区基因的体外扩增,克隆和序列分析

根据免疫球蛋白重链和轻链可变区基因５＇端序列和Ｊ区序列,化学合成适合于体外扩增抗体重、轻链可变区基因的二对引物。从体外培养的ＯＫＴ３杂交瘤细胞中提取总ＲＮＡ,反转录生成ｃＤＮＡ,以ｃＤＮＡ为模板,分别加入合成的重、轻链可变区引物进行ＰＣＲ,扩增出抗体重、轻链可变区基因片段。将扩增产物分别插入ｐＵＣ１９质粒,筛选出阳性克隆,用链终止法进行ＤＮＡ序列测定。所测重链可变区基因全长３５７ｂｐ,编码１１９个     

汉坦病毒陈株S基因编码区的克隆,序列分析及表达

从汉坦病毒陈株感染的ＶｅｒｏＥ６细胞裂解液中提取病毒ＲＮＡ,经逆转录ＰＣＲ获得病毒Ｓ基因编码区约１．３ｋｂｃＤＮＡ片段,克隆该片段后进行核苷酸序列测定,并与汉坦病毒７６１１８株进行同源性比较,结果二者核苷酸序列同源性为８６％,推导的氨基酸序列同源性为９７％。将该基因片段插入原核表达载体ｐＧＥＸ４Ｔ１,在大肠杆菌中获得高效表达。表达产物为ＧＳＴＮＰ融合蛋白。ＳＤＳＰＡＧＥ检测表达蛋白分子约７２ｋＤ左右。Ｗｅｓｔｅｒｎｂｌｏｔｉｎｇ和ＥＬＩＳＡ试验结果表明,表达产物可与多株抗汉坦病毒核蛋白的ＭｃＡｂ发生反应,其抗原表位及ＭｃＡｂ反应谱与７６１１８株相比存在某些差异。     

抗人CD3单抗重、轻链可变区基因的体外扩增、克隆和序列分析

根据免疫球蛋白重链和轻链可变区基因５’端序列和Ｊ区序列,化学合成适合于体外扩增抗体重、轻链可变区基因的二对引物。从体外培养的ＯＫＴ３杂交瘤细胞中提取总ＲＮＡ,反转录生成ｃＤＮＡ,以ｃＤＮＡ为模板,分别加入合成的重、轻链可变区引物进行ＰＣＲ,扩增出抗体重、轻链可变区基因片段。将扩增产物分别插入ｐＵＣ１９质粒,筛选出阳性克隆,用链终止法进行ＤＮＡ序列测定。所测重链可变区基因全长３５７ｂｐ,编码１１９个氨基酸,轻链可变区基因全长３２１ｂｐ,编码１０７个氨基酸。     

中国人肥胖基因克隆及其原核表达载体的构建

为了探讨人肥胖（obesity,OB）基因的生理和病理意义,利用逆转录-聚合酶链式．反应（RT-PCR）方法,从中国汉族成人腹膜后脂肪组织总RNA中扩增出肥胖基因编码区序列（cDNA）．定向亚克隆pUC19质粒,克隆的OBcDNA不含信号肽序列并加入了新的起始密码子ATG,序列分析表明,与日本报道的人OBcDNA相比,多出一个谷氨酸密码子CAG．将OBcDNA定向克隆至原核表达载体pBV220,构建了重组OB基因表达质粒pBV220-OB．SDS-PAGE证实pBV220-OB在大肠杆菌中可表达分子量为16.7KD的特异蛋白带．     

大鼠μ型阿片受体的pIRES2-EGFP质粒构建及其在HEK293细胞中的表达

提取大鼠脑组织总RNA,通过逆转录巢式PCR,扩增μ型阿片受体全长cDNA,克隆至pMD20-T载体中,测序鉴定,纠正点突变后,经酶切连接克隆入pIRES2-EGFP中,测序及酶切结果表明μ基因正确,μ-pIRES2-EGFP质粒构建成功.用脂质体法将μ-pIRES2-EGFP转染入HEK293细胞中,在荧光显微镜下,转染细胞可以观察到绿色荧光,应用免疫组化荧光可以观察到μ基因的高强度表达.     

Comparison of cDNA and genomic forms of tyrosine hydroxylase gene therapy of the brain with Trojan horse liposomes

BACKGROUND: The present study examines whether chromosomal derived forms of therapeutic genes can be delivered to brain following intravenous administration. The brain expression of a rat tyrosine hydroxylase (TH) cDNA is compared to the brain expression of a plasmid DNA encoding the 18 kb rat TH gene. METHODS: TH gene expression is measured in cell culture and in vivo in brain in experimental Parkinson's disease (PD). A total of four eukaryotic expression plasmids encoding rat TH were engineered wherein the size of the TH expression cassette ranged from 1.5 kb, in the case of the cDNA form of the gene, to 17.5 kb, in the case of the largest size genomic construct. The TH expression plasmids were delivered to either cultured cells or to rat brain in vivo with Trojan horse liposomes (THLs), which target the non-viral plasmid DNA to cells via cell membrane receptors. RESULTS: The pattern of TH gene expression in cell culture and in vivo was similar: the cDNA form of the TH gene was fast-acting with short duration of action, and the genomic form of the TH gene was slow-acting with longer duration of action. The most sustained replacement of striatal TH enzyme activity in experimental PD was produced by combination gene therapy where both the cDNA and the genomic forms of the TH gene were administered simultaneously. CONCLUSIONS: Eukaryotic expression plasmids encoding genomic forms of therapeutic genes, as large as 18 kb, can be successfully incorporated in THLs and delivered to brain following intravenous administration.     

拯救细胞系恢复重组家蚕核型多角体病毒包涵体实现外源蛋白在家蚕中产业化生产

构建家蚕Bombyx mori肌动蛋白（BmA3）启动子驱动的家蚕核型多角体病毒（BmNPV）多角体基因（ph）和OpNPV极早期启动子（IE1）驱动的zeocin抗性筛选基因转座供体载体,与鳞翅目辅助转座质粒pie2piggyBac共转染家蚕卵巢细胞BmN,经200μg/ml zeocin抗生素筛选一个月,成功获得持续表达BmNPV多角体蛋白的稳定细胞系BmN-A3ph。多角体缺陷型重组病毒BmBac-GF P感染拯救细胞系BmN- A3ph, 细胞成功装配出病毒包涵体颗粒,其包装效率约为野生型病毒感染正常BmN细胞的8%。用拯救型包涵体病毒颗粒喂食家蚕幼虫进行复感染,结果表明稳定细胞系所包装的包涵体病毒与野生型病毒一样能够通过口服途径感染宿主,却并不在宿主体内形成包涵体,从而保证外源基因高效表达。拯救型包涵体病毒可望解决传统注射感染效率较低问题,通过喂食感染可促进杆状病毒介导的家蚕生物反应器产业化进程。     

一条大鼠睾丸新基因的生物信息学分析及真核表达

目的:探讨大鼠睾丸组织一条新基因的生物信息学特征和真核表达。方法:构建pEGFP-N1载体的融合质粒进行真核表达,利用生物信息学手段分析基因和蛋白功能。结果:生物信息学分析表明RSA14-44的编码区序列与人类及鼠源RAS同源基因家族核酸序列达到85%以上的同源性;RSA14-44蛋白没有典型的跨膜结构域,也没有典型的N末端信号肽;与人类RhoA蛋白序列达到了89%的同源且具有Rho家族成员的GAAX盒和p-loop结构的基序特征;RSA14-44蛋白大部分氨基酸序列与Rho家族7个已知结构域高度同源;RSA14-44基因真核表达定位于细胞质。结论:RSA14-44基因真核表达定位于CHO-K1细胞质,;编码蛋白质与Rho家族同源性高,为进一步研究其生物学功能提供参考。     

大鼠α-酰胺酶在变铅青链霉菌中的克隆及表达研究

α－酰胺酶（α－ａｍｉｄａｓｅ,α－ＡＥ）催化神经和内分泌系统中活性多肽的Ｃ－端酰胺化,多多肽的生物活性至关重要。以大鼠心房组织的总ＲＮＡ为模板,采用ＲＴ－ＰＣＲ技术扩增获得编码α－酰胺酶的ｃＤＮＡ,并进行了克隆和测序。为了使α－酰胺酶能在链霉菌中分泌表达,将其ｃＤＮＡ与链霉菌酷氮酶酶（ｍｅｌＣ１）信号的编码序列融合得到融合ｍｅｌ／ＡＥ,将ｍｅｌ／ＡＥ插入链霉菌质粒ｐＩＪ６８０,获得重组质粒ｐＩＪ     

The repetitive structure of the profilaggrin gene as demonstrated using epidermal profilaggrin cDNA

Filaggrin is the histidine-rich basic protein that aggregates keratin filaments in fully differentiated cells of the epidermis. Filaggrin is synthesized in the granular cell layer as a high molecular weight precursor protein (profilaggrin) that consists of multiple repeated copies of filaggrin. cDNA clones for rat and mouse epidermal profilaggrin have been constructed from sucrose gradient-enriched RNA in order to study the repetitive structure of profilaggrin. These clones hybridize to high molecular weight epidermal mRNA (23 kilobase pairs, rat and 19 kilobase pairs, mouse) and exhibit limited cross-hybridization between species. Several rat clones direct the synthesis of a portion of rat profilaggrin in bacteria. One of these, rat profilaggrin cDNA clone R4D6, is 2400 base pairs in length. The R4D6 cDNA is shown to contain repetitive sequence by restriction mapping and southern hybridization analysis of restriction digests of this plasmid, using subfragments of the plasmid as hybridization probes. Southern hybridization analysis of rat genomic DNA, digested to completion with several restriction enzymes, reveals a simple hybridization pattern of fragments equal in size to those of the cDNA. Partial digestion of rat genomic DNA results in a ladder of bands based on a 1200-base pair repeat, equal to the size of the repeating unit of the cDNA clone, and consistent with the expected repeating size of profilaggrin. Together, these results show that the profilaggrin mRNA and gene have repetitive structure and that the gene apparently lacks introns in the coding region.     

Expression of the genes coding for the skeletal muscle and cardiac actions in the heart

Several types of evidence indicate that the gene coding for the skeletal muscle actin is expressed in the rat heart: 1) A recombinant plasmid containing an insert with a nucleotide sequence identical to that of the homologous region of skeletal muscle actin gene was isolated from a cDNA library prepared on rat cardiac mRNA template. 2) Using specific probes it was found that the hearts of newborn rats contain a significant amount of skeletal muscle actin mRNA. The quantity of this mRNA in the heart decreases during development. 3) The skeletal muscle actin gene is DNAase I sensitive in nuclei from rat heart tissue. A plasmid containing a cDNA insert homologous to a part of the cardiac actin mRNA was isolated and sequenced. It was found that in spite of the great similarity between the amino acid sequence of the skeletal muscle and cardiac actins, the nucleotide sequences of the two mRNAs are considerably divergent. There is only limited sequence homology between the 3' untranslated regions of the two mRNAs. However, there is an extensive sequence homology between the 3' untranslated regions of the rat and human cardiac mRNAs, suggesting a functional role for this region of the gene or mRNA.