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1.
红曲霉原生质体的制备、再生及其遗传转化系统 总被引:14,自引:1,他引:13
原生质体是研究和建立真菌遗传转化系统的重要工具。为了建立原生质体介导的红曲霉遗传转化系统,考察了各种细胞壁裂解酶和渗透压稳定剂等对红曲霉原生质体形成和再生的影响。将红曲霉分生孢子在铺有玻璃纸的平板上30℃培养30~40 h收获的菌丝体最有利于原生质体的形成和释放。红曲霉菌丝体形成和释放原生质体最适裂解酶和酶解时间分别为:0.3 % lysing enzyme、0.1 % cellulase和1 % snailase的酶组合,30℃作用2.5 h;最适渗透压稳定剂是:1mol /L MgSO4。最适合原生质体再生的培养基为含0.6 mol/L蔗糖的CM培养基。原生质体液涂布单层再生培养基的方法,再生率最高,菌株M34和N18分别为8.5 %和36.4 %。在PEG和CaCl2存在下,以潮霉素B为抗生素选择标记,用质粒pBC-Hygro和pNL1共转化菌株M34原生质体,每微克DNA克获得100个稳定转化子。 相似文献
2.
用Bio-Rad生产的基因脉冲仪进行酿酒酵母电击转化实验,得到的最适条件为:5kv/cm25μF和200Ω。电击后涂布前的培养时间为2小时。电击后细胞存活率为46%时,每微克质粒DNA得到106以上的转化子。用相同的质粒和受体菌进行原生质体法和醋酸锂法比较实验,转化率分别为2×104和3.5×102个转化子/μgDNA。电击转化是最方便易行和高效率的方法。 相似文献
3.
为从分子水平上阐释产甘油假丝酵母(Candida glycerinogenes)高产甘油机理,建立一种方便可行的遗传转化系统是十分必要的。与G418和潮霉素等抗生素相比,Zeocin抗生素对C.glycerinogenes具有较低的致死浓度。以pGAPZb作为构建整合载体的骨架,以Zeocin抗性基因作为选择标记,以URA3基因作为整合位点,构建了C.glycerinogenes整合载体pGA-CU。整合载体经过限制酶线性化后用作转化载体,基于电击转化的方法成功获得了抗Zeocin的转化子并经过PCR分析进一步确证。通过优化电击转化的参数,获得了较为稳定的转化效率,基于这一技术的转化效率每微克DNA可获得120个转化子。为进一步研究该菌株的遗传背景和代谢机理奠定了基础。 相似文献
4.
为了建立适合米根霉的遗传转化体系,应用重叠延伸PCR的方法构建了以潮霉素B抗性为选择标记的单交换整合型表达载体p BS-hygro-ldh A;分别采用PEG/Ca Cl2介导的原生质体转化、原生质体电转化及萌发孢子电转化的方法将表达载体p BS-hygro-ldh A转化入米根霉AS 3.819菌株中,并研究了菌丝酶解时间、孢子萌发时间以及电转化电场强度对于转化效率的影响;通过荧光定量PCR(q PCR)对米根霉转化子基因组中质粒整合拷贝数进行了检测,并研究了其对米根霉转化子抗性稳定性的影响。实验结果表明成功获得整合了表达载体p BS-hygro-ldh A的米根霉转化子。菌丝酶解140 min产生的原生质体其再生率和转化率最高,原生质体电转化最佳电场强度为13 k V/cm,孢子萌发2.5 h转化率最高,萌发孢子电转化最佳电场强度为14 k V/cm。萌发孢子电转化方法转化率要高于原生质体转化的方法。荧光定量PCR检测结果表明,在一定范围内,高质粒整合拷贝数的米根霉转化子比较稳定。研究建立了用于工业米根霉菌株的遗传转化体系,为米根霉代谢调控研究以及菌种改造工作提供了基础与支持。 相似文献
5.
采用PEG介导的原生质体转化方法,研究了将含有潮霉素抗性基因的质粒pMP-Hygro转入红曲菌9903A的影响因素。实验结果表明,原生质体转化最佳条件为:1.0mol/L的山梨醇为渗透压稳定剂;以含有50mmol/L的Ca2 和最终质量分数为40%的PEG4000为转化介质;最佳原生质体浓度和载体DNA用量分别为1×108个/mL、1μg/100μL原生质体;原生质体再生培养基采用不含无机盐的培养基,再生方式采用原生质体液涂布单层再生培基平板法。得到的平均DNA转化率可达160个/μgDNA。本文所研究的PEG介导的原生质体转化方法可以较好的向红曲菌细胞导入外源DNA,并使外源DNA在红曲菌细胞内大量表达。 相似文献
6.
为了分离耐高渗和甘油代谢相关基因,以Zeocin为选择标记,利用REMI技术电转化产甘油假丝酵母Candida glycerinogenes。考察了7种限制性内切酶对转化的影响,选择HindIII进一步优化了转化的几个条件。结果表明,在OD600≈1.3时收集细胞,在1.5kV电压下,感受态细胞浓度为2.0×109个细胞/mL,100U Hind III时,能获得129个转化子/μgDNA的较高转化率,58%的转化子稳定,表明REMI技术适合于产甘油假丝酵母的转化。 相似文献
7.
摘要:【目的】在球毛壳菌(Chaetomium globosum)NK-102 中,建立菌株特异性转化体系。【方法】构建新的抗性标记pUCATPH-Pgap,转化效率优于pUCATPH 和pCM768。建立了PEG-原生质体和根癌农杆菌(Agrobacterium tumefaciens)EHA105 介导的两种转化方法。【结果】原生质体转化效率为30-50 个转化子/10 μg DNA,抗性标记pUCATPH-Pgap 效率最高。EHA105 介导转化率达到3.2×102 转化子/107 孢子。Sout 相似文献
8.
为从分子水平上阐释产甘油假丝酵母(Candida glverinogenes)高产甘油机理,建立一种方便可行的遗传转化系统是十分必要的。与G418和潮霉素等抗生素相比,Zeoein抗生素对C.glycerinogenes具有较低的致死浓度。以pGAPZb作为构建整合载体的骨架,以Zeocin抗性基因作为选择标记,以URA3基因作为整合位点,构建了C.glycerinogenes整合载体pGA-CU。整合载体经过限制酶线性化后用作转化载体,基于电击转化的方法成功获得了抗Zeocin的转化子并经过PCR分析进一步确证。通过优化电击转化的参数,获得了较为稳定的转化效率,基于这一技术的转化效率每微克DNA可获得120个转化子。为进一步研究该菌株的遗传背景和代谢机理奠定了基础。 相似文献
9.
10.
农杆菌介导的紫色红曲霉遗传转化体系的建立和优化 总被引:1,自引:0,他引:1
通过优化各种转化因素,建立了根癌农杆菌(Agrobacterium tumefaciens)介导红曲霉(Monascus)的高效转化体系:红曲霉在PDA培养基培养21 d后收集孢子,制备红曲霉孢子悬浮液,浓度为106个/mL,根癌农杆菌浓度为OD600值0.5,诱导剂AS浓度为100μmol/L,农杆菌与红曲霉在25℃共培养3 d。采用此转化体系构建了含有530多个转化子的红曲霉T-DNA插入突变体库。随机选取50株转化子菌株进行分子验证和稳定性检测,证明T-DNA成功插入红曲霉基因组DNA中,并能稳定遗传。最后,通过形态观察筛选出8株变异较大的菌株,为以后的红曲霉基因功能研究奠定了一定的基础。 相似文献
11.
J. S. Brown A. Aufauvre-Brown D. W. Holden 《Molecular genetics and genomics : MGG》1998,259(3):327-335
We have investigated transformation with heterologous DNA as a method for insertional mutagenesis of Aspergillus fumigatus. Two methods, polyethylene glycol-mediated transformation of protoplasts and electroporation of germinating spores, were used to establish conditions leading to single-copy integration of transforming DNA at different genomic sites. We have assessed the effect of restriction enzyme-mediated integration (REMI) for both methods. Non-REMI protoplast transformation led to integration of multiple copies of transforming DNA in the majority of transformants. Results of REMI with protoplast transformation varied depending on the enzyme used. Low concentrations of several restriction enzymes stimulated transformation, but of ten enzymes investigated only REMI with XhoI and KpnI resulted in single-copy integration of transforming DNA for the majority of transformants. For protoplast transformation with XhoI- or KpnI-based REMI, 50% and 76% of insertions, respectively, were due to integrations at a genomic enzyme site corresponding to the enzyme used for REMI. Electroporation of spores without addition of restriction enzyme resulted in a high transformation efficiency, with up to 67% of transformants containing a single copy of transforming DNA. In contrast to protoplast transformation, electroporation of spores in the presence of a restriction enzyme did not improve transformation efficiency or lead to insertion at genomic restriction sites. Southern analysis indicated that for both protoplast transformation with REMI using KpnI or XhoI and for electroporation of spores without addition of restriction enzymes, transforming DNA inserted at different genomic sites in a high proportion of transformants. 相似文献
12.
We have investigated transformation with heterologous DNA as a method for insertional mutagenesis of Aspergillus fumigatus. Two methods, polyethylene glycol-mediated transformation of protoplasts and electroporation of germinating spores, were
used to establish conditions leading to single-copy integration of transforming DNA at different genomic sites. We have assessed
the effect of restriction enzyme-mediated integration (REMI) for both methods. Non-REMI protoplast transformation led to integration
of multiple copies of transforming DNA in the majority of transformants. Results of REMI with protoplast transformation varied
depending on the enzyme used. Low concentrations of several restriction enzymes stimulated transformation, but of ten enzymes
investigated only REMI with XhoI and KpnI resulted in single-copy integration of transforming DNA for the majority of transformants. For protoplast transformation
with XhoI- or KpnI-based REMI, 50% and 76% of insertions, respectively, were due to integrations at a genomic enzyme site corresponding to
the enzyme used for REMI. Electroporation of spores without addition of restriction enzyme resulted in a high transformation
efficiency, with up to 67% of transformants containing a single copy of transforming DNA. In contrast to protoplast transformation,
electroporation of spores in the presence of a restriction enzyme did not improve transformation efficiency or lead to insertion
at genomic restriction sites. Southern analysis indicated that for both protoplast transformation with REMI using KpnI or XhoI and for electroporation of spores without addition of restriction enzymes, transforming DNA inserted at different genomic
sites in a high proportion of transformants.
Received: 6 March 1998 / Accepted: 25 May 1998 相似文献
13.
Use of REMI and Agrobacterium-mediated transformation to identify pathogenicity mutants of the biocontrol fungus, Coniothyrium minitans 总被引:7,自引:0,他引:7
Restriction enzyme mediated integration (REMI) and Agrobacterium-mediated transformation (ATMT) were used to transform protoplasts or germinated conidia of the mycoparasite Coniothyrium minitans to hygromycin resistance. Using REMI, up to 32 transformants mug DNA(-1) were obtained, while 37.8 transformants 5 x 10(5) germlings(-1) were obtained using ATMT. Single-copy integrations occurred in 8% and 40% of REMI and ATMT transformants, respectively. A novel microtitre plate-based test was developed to expedite screening of 4000 REMI and ATMT C. minitans transformants. Nine pathogenicity mutants that displayed reduced or no pathogenicity on sclerotia of Sclerotinia sclerotiorum were identified. 相似文献
14.
The techniques of restriction enzyme-mediated integration (REMI) and electroporation (EP) were applied for the first time to improving the blastospore transformation of fungal biocontrol agent Beauveria bassiana for higher frequency. The blastospores from < or =24 h incubation in glucose-mineral medium after shaking conidia for 48 h in Subouraud dextrose broth were found most competent for integrating 1 microg plasmid DNA vectoring the phosphinothricin (PPT) resistance gene bar in 360 microL reaction system containing 100 U HindIII or XbaI. Such blastospores were also most suitable for EP transformation at the optimized field strength of 10 kV cm(-1). The optimized REMI and EP generated averagely 39 and 53 transformants microg(-1) plasmid DNA whereas polyethylene glycol (PEG) integration yielded only 22. All transformants grew well on Czapek's agar containing 400 microg PPT mL(-1) after three rounds of cultivation on the same agar excluding PPT but their parental strain showed no resistance. The target gene inserted into the genomes of 10 transformants randomly taken from REMI or EP transformation was consistently detected by both PCR and Southern blotting. Compared to the PEG integration, REMI and EP enhanced the frequency of the blastospore transformation by 73 and 137%, respectively. 相似文献
15.
《Bioscience, biotechnology, and biochemistry》2013,77(12):2224-2227
A new rapid transformation system for Aspergillus niger that uses electroporation to render intact germinating conidia permeable to DNA is described. The transformant colonies appeared earlier than transformants obtained by the protoplast-forming method. Without pretreatment of the conidia the transformation frequencies were 1.2 colonies per μg of integrative vector and 100 colonies per μg of plasmid DNA. When the conidia were treated with a dilute solution of fungal cell wall lytic enzyme, the frequency of transformation was increased by approx. 2-fold when using two vectors. Southern blot analysis of genomic DNA and restriction endonuclease-digested DNA from a random sample of transformants showed homologous and nonhomologous integration of the integrative vector into the genome, as is also observed with the protoplast-forming method. In transformation with the plasmid vector, the transformant DNA was shown to be mostly maintained in free form with minimal integration into the chromosome when transformed by either intact electroporation or the conventional method. 相似文献
16.
We have used a plasmid containing the argB gene to transform an Aspergillus nidulansargB-deleted strain in the presence of restriction enzymes and show a 20- to 60-fold increase in transformation frequency via restriction enzyme-mediated integration (REMI). This procedure was used to try to tag new genes involved in the asexual development of this fungus. More than 2000 transformants isolated following electroporation of conidia and ~3700 transformants recovered following protoplast fusion were screened for sporulation defects. Unexpectedly, developmental mutants were obtained only when the protoplast fusion approach was used. Southern blot analysis of these mutants, and of randomly selected transformants obtained by electroporation, was consistent with the occurrence of single plasmid integration events in 33 and 65% of the cases, respectively. The argB marker was shown to be tightly linked to the mutant phenotype in only 62% of the mutants analyzed by sexual crosses. Partial DNA sequencing of a tagged gene, whose mutation delays asexual sporulation and results in a fluffy phenotype, showed no homology to previously reported sequences. Our results indicate that REMI can be used in A.?nidulans to increase the transformation frequency and illustrate the advantages and potential problems when using REMI to tag genes of interest in this and other fungi. 相似文献
17.
《Molecular & general genetics : MGG》1998,258(1-2):89-94
We have used a plasmid containing the argB gene to transform an Aspergillus nidulansargB-deleted strain in the presence of restriction enzymes and show a 20- to 60-fold increase in transformation frequency via
restriction enzyme-mediated integration (REMI). This procedure was used to try to tag new genes involved in the asexual development
of this fungus. More than 2000 transformants isolated following electroporation of conidia and ∼3700 transformants recovered
following protoplast fusion were screened for sporulation defects. Unexpectedly, developmental mutants were obtained only
when the protoplast fusion approach was used. Southern blot analysis of these mutants, and of randomly selected transformants
obtained by electroporation, was consistent with the occurrence of single plasmid integration events in 33 and 65% of the
cases, respectively. The argB marker was shown to be tightly linked to the mutant phenotype in only 62% of the mutants analyzed by sexual crosses. Partial
DNA sequencing of a tagged gene, whose mutation delays asexual sporulation and results in a fluffy phenotype, showed no homology
to previously reported sequences. Our results indicate that REMI can be used in A. nidulans to increase the transformation frequency and illustrate the advantages and potential problems when using REMI to tag genes
of interest in this and other fungi.
Received: 22 August 1997 / Accepted: 20 November 1997 相似文献
18.
Transformation of taxol-producing endophytic fungi by restriction enzyme-mediated integration (REMI) 总被引:1,自引:0,他引:1
The REMI method was used to introduce the plasmid pV2 harboring the hygromycin B phosphotransferase (hph) gene controlled by the Aspergillus nidulans trpC promoter and the trpC terminator into a taxol-producing endophytic fungus BT2. REMI transformation yielded stable transformants capable of continuing to grow on PDA medium containing 125 mug mL(-1) hygromycin B. The transformation efficiency was about 5-6 transformants mug(-1) plasmid DNA. The presence of hph gene in transformants was confirmed by PCR and Southern blot analyses. To the authors' knowledge, this is the first report on the transformation of taxol-producing endophytic fungi by the REMI technique. This study provides an effective approach for improving taxol production of endophytic fungi by the genetic engineering of taxol biosynthetic pathway genes in the future. 相似文献