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A transformation system for the yeast Candida utilis: use of a modified endogenous ribosomal protein gene as a drug-resistant marker and ribosomal DNA as an integration target for vector DNA.

机译：酵母假丝酵母的转化系统：使用修饰的内源核糖体蛋白基因作为抗药性标记，使用核糖体DNA作为载体DNA的整合靶标。

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We have developed a transformation system for the yeast Candida utilis. A novel strategy was applied to construct the transformation system, since auxotrophic mutants which could be used as hosts for transformation are not available. A gene encoding the ribosomal protein L41 was cloned from C. utilis, which is sensitive to cycloheximide, and used as a marker gene conferring cycloheximide resistance after modification of its amino acid sequence. The marker gene was constructed by substitution of the proline codon at position 56 with the glutamine codon by in vitro mutagenesis, as it had been reported previously that the 56th amino acid residue of L41 is responsible for the cycloheximide sensitivity of various organisms (S. Kawai, S. Murao, M. Mochizuki, I. Shibuya, K. Yano, and M. Takagi, J. Bacteriol. 174:254-262 1992). The ribosomal DNA (i.e., DNA coding for rRNA) of C. utilis was also cloned and used as a multiple-copy target for the integration of vector DNA into the genome, which resulted in a high transformation efficiency. Transformants were obtained by electroporation with a maximum efficiency of approximately 1,400 transformants per 1 microgram of linearized DNA carrying the gene for cycloheximide resistance and part of the ribosomal DNA. No transformants were obtained with intact plasmids. Multiple copies of the linearized plasmid were integrated into the host chromosome by homologous recombination. Southern analysis of the transformants in which vector DNA was integrated at the L41 gene locus indicated that there are two copies of gene for the L41 protein per cell, suggesting that C. utilis is diploid. Transformants were obtained from a variety of C. utilis strains, indicating that this method is applicable to the transformation of other C. utilis strains, even though there is significant heterogeneity in chromosomal karyotypes among these strains.

机译：我们已经开发了一种酵母菌假丝酵母的转化系统。由于无法获得可以用作转化宿主的营养缺陷型突变体，因此采用了一种新颖的策略来构建转化系统。从对毛环己酰亚胺敏感的C.utilis克隆编码核糖体蛋白L41的基因，并在其氨基酸序列修饰后用作赋予环己酰亚胺抗性的标记基因。标记基因是通过体外诱变通过用谷氨酰胺密码子取代第56位的脯氨酸密码子而构建的，因为以前已经报道过，L41的第56个氨基酸残基负责各种生物对环己酰亚胺的敏感性（S. Kawai ，S。Murao，M。Mochizuki，I。Shibuya，K。Yano，和M. Takagi，J。Bacteriol。174：254-262 1992）。还克隆了鱼梭菌的核糖体DNA（即，编码rRNA的DNA），并将其用作将载体DNA整合到基因组中的多拷贝靶标，这导致了高转化效率。通过电穿孔以每1克带有环己酰亚胺抗性基因和部分核糖体DNA的线性化DNA的最大效率约为1400个转化体获得转化体。用完整质粒没有获得转化体。通过同源重组将多个拷贝的线性化质粒整合到宿主染色体中。在L41基因位点整合了载体DNA的转化子的Southern分析表明，每个细胞中有两个L41蛋白的基因拷贝，这表明鱼C. utilis是二倍体。从多种C. utilis菌株获得了转化体，表明该方法适用于其他C. utilis菌株的转化，即使这些菌株的染色体核型存在显着的异质性。

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Kondo, K; Saito, T; Kajiwara, S; Takagi, M; Misawa, N;
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年度 1995
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1. A transformation system for the yeast Candida utilis: use of a modified endogenous ribosomal protein gene as a drug-resistant marker and ribosomal DNA as an integration target for vector DNA. [J] . K Kondo, T Saito, S Kajiwara, Journal of bacteriology . 1995,第24期

机译：酵母假丝酵母的转化系统：使用修饰的内源核糖体蛋白基因作为抗药性标记，使用核糖体DNA作为载体DNA的整合靶标。
2. Identification of a Candida utilis gene encoding ribosomal protein L7: evidence for two divergent subclasses of the eukaryotic ribosomal protein L7 family [J] . Nucleic acids research . 1993,第15期

机译：鉴定编码核糖体蛋白L7的鹦鹉螺假丝酵母基因：真核生物核糖体蛋白L7家族两个不同亚类的证据
3. Development of an integrative DNA transformation system for the yeast Candida utilis [J] . Rodriguez L., Basabe L., Rivero T., FEMS Microbiology Letters . 1998,第2期

机译：酵母菌假丝酵母的综合DNA转化系统的开发
4. CDNA and genomic sequence clonging and analysis of ribosomal protein L10A gene (RPL10A) from giant panda [C] . Zi-Mao Liu, Hou Yi-Ling, Xiang Ding, International Conference on Computer Science and Information Processing;CSIP 2012 . 2012

机译：大熊猫核糖体蛋白L10A基因（RPL10A）的CDNA和基因组序列延伸及分析
5. Phylogenetic analysis of brachionidae (phylum rotifera) using ribosomal DNA. [D] . Riva, Veronica de la. 1998

机译：利用核糖体DNA对腕足科（轮虫门）进行系统发育分析。
6. A transformation system for the yeast Candida utilis: use of a modified endogenous ribosomal protein gene as a drug-resistant marker and ribosomal DNA as an integration target for vector DNA. [O] . K Kondo, T Saito, S Kajiwara, 1995

机译：酵母假丝酵母的转化系统：使用修饰的内源核糖体蛋白基因作为抗药性标记使用核糖体DNA作为载体DNA的整合靶标。
7. Identification of a Candida utilis gene encoding ribosomal protein L7: evidence for two divergent subclasses of the eukaryotic ribosomal protein L7 family. [O] . Sharp, P M, Wolfe, K H 1993

机译：编码核糖体蛋白L7的假丝酵母基因的鉴定：真核生物核糖体蛋白L7家族两个不同亚类的证据。

A transformation system for the yeast Candida utilis: use of a modified endogenous ribosomal protein gene as a drug-resistant marker and ribosomal DNA as an integration target for vector DNA.

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