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1.
为了对酵母分子生物学理论研究及实际应用的探讨,进行了酵母DNA分子克隆。采用重组DNA技术及放射性分子探针杂交法从克隆库中检测出两大类含有ZDNA重复顺序的重组子。第一类是含有端粒区ZDNA重复顺序及自主复制顺序的重组子。这些重组子对端粒区灼整合转化研究对开拓基因工程的应用具有重要意义。第二类是含有染色体内部分散的ZDNA重复顺序的重组子。这些重组子对研究内在ZDNA的结构和功能有重要的理论价值。按实验结果计算,在酵母基因组中大约存在有100个ZDNA重复顺序片段。  相似文献   

2.
应用PCR技术从人胎肝cDNA库中扩增了人血管抑制素基因。将克隆的基因重组进酵母质粒pPIC9K获得含该基因的重组质粒pPIC9KA3。用电激法将质粒pPIC9K转化毕节酵母GSll5,经PCR检测获得含人血管抑制素基因的酵母工程菌GSll5(pPIC8KA3)。再用G418筛选法,在含不同浓度的G418平板上筛选高拷贝整合的转化子。对高拷贝整合的转化子进行发酵培养和诱导表达。SDS—PAGE及Westem印迹分析显示:表达产物约占胞外蛋白的43%,相当于94mg/L,并具有免疫活性。并能抑制bFGF诱导的鸡胚尿囊膜新生血管的生成。还对用G418筛选高拷贝整合转化子的方法做了探索。  相似文献   

3.
主要构建了可以与酵母染色体发生重组的质粒pAbAI-Bait,并转化大肠杆菌DH5α感受态细胞获得转化子,将阳性克隆进行PCR与DNA测序的方法鉴定,结果表明: 酵母单杂交中报告质粒pAbAI-Bait构建成功,可用于酵母单杂交体系.  相似文献   

4.
以重组质粒pcDNA6A-BMP6为模板PCR扩增hBMP6成熟肽cDNA编码序列,将该序列克隆到酵母分泌表达表达载体pPIC9K中.重组质粒pPIC9K-hBMP6经SacI酶切线性化,电击转化毕赤酵母GS115,PCR法筛选阳性转化子,利用梯度浓度G418筛选到七株高拷贝整合的阳性转化子。用甲醇进行诱导表达,SDSPAGE及Western-blot检测结果表明hBMP6成熟肽以分子量约为34和18 kD两种不同糖基化修饰的单体形式存在,具有良好的免疫原性.  相似文献   

5.
传统构建毕赤酵母质粒多拷贝菌株的方法不仅操作复杂、成本高,而且难以获得理想中的高拷贝菌株.近来,一种利用leu2-d缺陷型标记直接筛选毕赤酵母多拷贝克隆的方法显示出很大的便利.本研究发现,使用一个lys1-d缺陷型标记能更加高效地介导毕赤酵母超高拷贝质粒整合.首先构建一个携带lys1-d和EGFP(enhanced green fluorescent protein)报告基因的整合载体,然后将载体转化至敲除了内源lys1基因的毕赤酵母中,最后分别检测了转化子内EGFP含量和质粒拷贝数.结果显示,所有转化子整合的质粒拷贝数均处于19~168之间;并且转化子内质粒拷贝数越高,其胞内表达的EGFP产量也越高.这一系统为构建毕赤酵母超高拷贝质粒整合菌株增添了有效的工具.  相似文献   

6.
构建了编码汉坦病毒囊膜糖蛋白G2基因的重组质粒,在毕赤酵母中表达,为汉坦病毒基因工程疫苗的研究提供实验基础。利用PCR法从含汉滩病毒76-118株M基因的M56质粒中扩增编码糖蛋白G2的基因片段,克隆入酵母分泌表达载体pPICZαA,构建重组质粒pPICZαA-G2。酶切鉴定挑取的阳性克隆,转化入GS115工程菌,在含100μg/mLZeocin的YPD培养基上筛选。挑选单菌落,PCR鉴定阳性克隆,用0.5%甲醇诱导表达,并利用SDS-PAGE及Western-Blot鉴定表达产物。序列分析表明所获得的基因片段与编码汉滩病毒76-118株囊膜糖蛋白G2的基因一致;100μg/mLZeocinYPD培养基上筛选出含pPICZαA-G2转化子,PCR鉴定为阳性克隆;SDS-PAGE可见约70kDa处有目的蛋白表达条带,经Western-Blot证实该条带为汉滩病毒囊膜糖蛋白G2。成功地构建了重组酵母表达载体pPICZαA-G2,并在毕赤酵母中初步表达成功,为今后汉坦病毒囊膜糖蛋白G2表达纯化以及基因工程疫苗的制备奠定了一定基础。  相似文献   

7.
目的 :为用基因重组技术表达hCG避孕疫苗抗原 ,构建在酵母细胞中表达的重组质粒βhCG -pPIC9K ,转化嗜甲醇酵母 .方法 :根据βhCG的cDNA序列设计两条引物 ,使上游带EcoRI酶切位点 ,下游带NotI酶切位点 ,以质粒 βhCG -PBSKS为模板 ,进行PCR扩增反应 ;将所得的DNA片段经EcoRI和NotI双酶切后用T4连接酶与pPIC9K质粒进行连接 ,然后导入大肠杆菌DH5α ,用PCR筛选阳性克隆并用双酶切鉴定重组子βhCG -pPIC9K .再用电打孔法转化酵母 (Pichiapastoris) ,用缺组氨酸MD平板筛选阳性株并在含G4 18的YPD培养基中筛选多拷贝插入菌株 .结果 :用所设计的引物扩增出两端分别带EcoRI和NotI酶切位点的βhCGDNA片段 ,插入pPIC9K并导入DH5α获得阳性克隆 ,经PCR反应和双酶切鉴定表明重组质粒是 βhCG -pPIC9K ,并转化嗜甲醇酵母获得耐受 4mg/mLG4 18的菌株 .结论 :构建了重组质粒 βhCG -pPIC9K并获得插入重组质粒 βhCG -pPIC9K的嗜甲醇酵母  相似文献   

8.
家蝇防御素defensin cDNA的克隆及在毕赤酵母中的表达   总被引:6,自引:0,他引:6  
提取家蝇总RNA,RT-PCR扩增编码家蝇防御素defensin的cDNA,克隆并测定了其序列,将该cDNA序列与酵母表达载体pPICZαA重组,构建酵母分泌型表达载体pPICZα-de,电激法转化毕赤酵母(Pichia pasto-ris)受体菌GS115。经表型筛选和PCR鉴定证明目的片段已稳定整合到酵母染色体基因组中。在含不同浓度的Zeoc in平板上筛选到高拷贝整合的转化子,阳性克隆经甲醇诱导表达,用Tric ine-SDS-PAGE确定了表达产物的正确性,琼脂孔穴平板扩散法、比浊法测定了表达产物的活性,对金黄色葡萄球菌Staphylococcus aureus具有一定的杀菌活性。  相似文献   

9.
构建和转化神经营养素3(neurotrophin 3,NT3)的酵母诱饵重组质粒,为通过酵母双杂交研究NT3的功能及作用机制奠定基础。用PCR扩增NT3基因cDNA中编码完整开放读框的基因片段;将该基因片段与pLexA载体定向重组;用酶切和测序鉴定重组质粒;将核苷酸序列正确的重组质粒转化入EGY48[p8op LacZ]酵母菌株。结果成功构建pLexA NT3重组质粒。转化有重组质粒和pLexA空载体的二种EGY48[p8op LacZ]酵母都能在SD Gal Raf His Ura培养基中长成白色菌落(同时,转化pLexA pos阳性对照质粒的酵母菌在相同条件下长成蓝色菌落),但都不能在SD His Leu Ura培养基中生长,在SD His Ura液中培养16h后,OD600均值均为0.8±0.1。这表明,重组质粒表达的融合蛋白没有激活LEU2和lacZ酵母报告基因表达的活性,也没有酵母毒性作用。因此,构建的诱饵重组质粒可以用于下一阶段的人胎脑cDNA文库筛选。  相似文献   

10.
根据酵母整合质粒的设计要求,PCR扩增特定的2.2kb rDNA片段,并以此替换酿酒酵母(Saccharomyces cereristae)整合载体YIp5的URA3片段;在此基础上,引入G418抗性基因KanMX和酵母磷酸甘油激酶(phosphoglycerale kinase,PGK)组成型强启动子和终止子序列(PGKp-t),构建适合酿酒酵母工业菌株高拷贝整合表达载体pYMIKP,以细菌木糖异构酶(xylose isomerase,XI)基因xy/A为目标基因,通过载体pYMIKP引入到酵母工业菌株NAN-27中,酵母转化子在非选择培养条件下,连续生长50世代质粒稳定性为99.72%,目标基因高拷贝重组菌的木糖异构酶比酶活是对照菌株的67.2倍,达到0.672U/mg蛋白,实现了外源基因在酿酒酵母工业菌株中的稳定高效表达。  相似文献   

11.
Transformation of yeast by a replicating hybrid plasmid.   总被引:74,自引:0,他引:74  
J D Beggs 《Nature》1978,275(5676):104-109
Chimaeric plasmids have been constructed containing a yeast plasmid and fragments of yeast nuclear DNA linked to pMB9, a derivative of the ColEl plasmid from E. coli. Two plasmids were isolated which complement leuB mutations in E. coli. These plasmids have been used to develop a method for transforming a leu2 strain of S. cerevisiae to Leu+ with high frequency. The yeast transformants contained multiple plasmid copies which were recovered by transformation in E. coli. The yeast plasmid sequence recombined intramolecularly during propagation in yeast.  相似文献   

12.
An efficient transformation method mediated by PEG-protoplasts was developed for the newly commercial edible mushroom Pleu-rotus nebrodensis. Two plasmids were used to co-transform protoplasts of P. nebrodensis. One plasmid is pAN7-1 containing a positive selectable marker gene hph conferring hygromycin B resistance. Another plasmid is pBIue-GFP containing a reporter gene gfp conferring green fluorescent protein. PCR and Southern blot analysis showed that hph gene or/and gfp gene were integrated into the genome of P.nebrodensis transformants. The transformation efficiency of the positive selectable marker gene hph was 3 transformants per microgram of plasmid pAN7-1 DNA, which was about 30 times higher than that previously reported in thoroughly studied Pleurotus species such as Pleurotus ostreatus. The transformation efficiency of the reporter gene gfp was 9 transformants per microgram of plasmid pBlu-GFP DNA. The co-transformation efficiency was 23.68%. This is the first report that a "reporter" gene, green fluorescent protein gene can be successfully stably expressed in this Pleurotus species.  相似文献   

13.
S S Wang  V A Zakian 《Nature》1990,345(6274):456-458
DNA termini from Tetrahymena and Oxytricha, which bear C4A2 and C4A4 repeats respectively, can support telomere formation in Saccharomyces cerevisiae by serving as substrates for the addition of yeast telomeric C1-3A repeats. Previously, we showed that linear plasmids with 108 base pairs of C4A4 DNA (YLp108CA) efficiently acquired telomeres, whereas plasmids containing 28-64 base pairs of C4A4 DNA also promoted telomere formation, but with reduced efficiency. Although many of the C4A4 termini on these plasmids underwent recombination with a C4A2 terminus, the mechanism of telomere-telomere recombination was not established. We now report the sequence of the C4A4 ends from the linear plasmids. The results provide strong evidence for a novel recombination process involving a gene conversion event that requires little homology, occurs at or near the boundary of telomeric and nontelomeric DNA, and resembles the recombination process involved in bacteriophage T4 DNA replication.  相似文献   

14.
An efficient transformation method mediated by PEG-protoplasts was developed for the newly commercial edible mushroom Pleurotus nebrodensis. Two plasmids were used to co-transform protoplasts of P. nebrodensis. One plasmid is pAN7-1 containing a positive selectable marker gene hph conferring hygromycin B resistance. Another plasmid is pBlue-GFP containing a reporter gene gfp conferring green fluorescent protein. PCR and Southern blot analysis showed that hph gene or/and gfp gene were integrated into the genome of P. nebrodensis transformants. The transformation efficiency of the positive selectable marker gene hph was 3 transformants per microgram of plasmid pAN7-1 DNA, which was about 30 times higher than that previously reported in thoroughly studied Pleurotus species such as Pleurotus ostreatus. The transformation efficiency of the reporter gene gfp was 9 transformants per microgram of plasmid pBlu-GFP DNA. The co-transformation efficiency was 23.68%. This is the first report that a "reporter" gene, green fluorescent protein gene can be successfully stably exoressed in this Pleurotus species.  相似文献   

15.
~~甲醇酵母PEG和电转化法@李亚东$河北大学生命科学学院!河北保定071002 @王会文$河北大学生命科学学院!河北保定071002 @赵晓瑜$河北大学生命科学学院!河北保定071002~~~~~~  相似文献   

16.
黑曲霉(Aspergillus niger)具有高效的蛋白表达和分泌能力.为实现异源蛋白在无孢黑曲霉中的高效重组表达,在优化遗传筛选标记的基础上,建立了根癌农杆菌介导的、以潮霉素抗性基因为筛选标记的黑曲霉转化体系.利用该体系介导米黑根毛霉脂肪酶(RML)转化黑曲霉SH-1,通过PCR鉴定、酶活检测、镍柱亲和层析及SDS-PAGE电泳检测等确定成功获得了RML的黑曲霉转化子,并通过发酵条件优化实现了RML的高效表达,对硝基苯酚比色法测得转化子酶活最高可达15 U/mL,是其在酵母中表达水平的10倍以上.  相似文献   

17.
将乙型肝炎表面抗原基因组装进穿梭质粒,经E.coli扩增、鉴定后转入酵母细胞得到了转化子。经放射免疫分析,在此转化子中HBsAg未得到表达,可能是阅读框架不一致造成的。此外,我们对酵母DNA重组技术进行了摸索,并简化和改进了一些步骤。  相似文献   

18.
利用根癌农杆菌介导的转化方法改良木霉菌   总被引:3,自引:1,他引:3  
根癌农杆菌介导的转化系统在丝状真菌的研究中具有重要的意义。通过农杆菌介导,成功实现了丝状真菌绿色木霉菌(Trichoderma viride)遗传转化,转化率约为30~80个转化子/10^5个孢子。PCR检测和几丁质酶分析表明含有编码几丁质酶外源基因(Cli 113)的T-DNA已整合进木霉菌基因组中,而且转化子都能够稳定遗传。农杆菌介导的遗传转化方法具有转化率高、操作简便、遗传稳定等优点,在丝状真菌的遗传转化中具有重要的意义。  相似文献   

19.
利用根癌农杆菌LBA4404介导,建立了丝状真菌简青霉(Penicillium simpli-cissimum)H5的遗传转化系统.潮霉素抗性筛选、PCR和Southern blot分子鉴定等结果表明:筛选获得的转化子能够稳定遗传,外源的T-DNA以单拷贝随机整合到简青霉的基因组中.实验初步研究了农杆菌浓度、乙酰丁香酮浓度和共培养时间等因素对转化效率的影响,经过优化后转化体系的效率可达50个转化子/105个孢子.农杆菌介导的遗传转化方法在简青霉上的运用,将为研究该菌的基因工程改造提供强有力的工具.  相似文献   

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