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Cloning and Prokaryotic Expression of FnBP Ligand Binding Gene of Staphylococcus aureus 被引量:3
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作者 尹荣兰 杨正涛 +5 位作者 张艳晶 刘辉 刘珊 杨琦 曹永国 张乃生 《Agricultural Science & Technology》 CAS 2008年第6期43-46,共4页
[Objective] The study aimed to clone the FnBP ligand binding gene of Staphylococcus aureus and run prokaryotic expression by constructing a prokaryotic expression vector. [Method] The gene encoding FnBP ligand binding... [Objective] The study aimed to clone the FnBP ligand binding gene of Staphylococcus aureus and run prokaryotic expression by constructing a prokaryotic expression vector. [Method] The gene encoding FnBP ligand binding gene was amplified from S.aureus chromosomal DNA by PCR technique. After T-A cloning, plasmid pMD18- FnBP was constructed. pMD18- FnBP and pET28a(+)were digested by BamH Ⅰ and EcoR Ⅰ double enzymes, then the purified FnBP ligand binding gene was subcloned into the expression vector pET28a(+), and the prokaryotic expression vector pET28a-FnBP was thus constructed. The constructed plasmid pET28a-FnBP was transformed into Escherichia coli BL21(DE3) competent cells. The bacterium was induced by IPTG and the expressed products were analyzed by SDS-PAGE and Western blot. [Result] The gene fragment with the length of 370 bp was amplified by PCR approach. One approximately 30 kD exogenous protein was observed in SDS-PAGE analysis. Western blot analysis indicates the protein has antigenicity of S.aureus. [Conclusion] The FnBP ligand binding gene of S.aureus was successfully cloned and expressed in prokaryotic cells. 展开更多
关键词 STAPHYLOCOCCUS aureus FNBP ligand binding gene cloning prokaryotic expression
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Cloning and Prokaryotic Expression of NS1 Gene of Porcine Parvovirus (PPV) SD1 Strain 被引量:1
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作者 谢金文 沈志强 +3 位作者 王金良 任艳玲 管宇 苗立中 《Agricultural Science & Technology》 CAS 2007年第3期59-63,共5页
[Objective] The research aimed to provide the theoretical basis for establishing a rapid diagnosis method for porcine parvovirus(PPV). [ Method] One pair of primers were designed according to PPV genome sequences on... [Objective] The research aimed to provide the theoretical basis for establishing a rapid diagnosis method for porcine parvovirus(PPV). [ Method] One pair of primers were designed according to PPV genome sequences on GenBank website and the sequences of prokaryotic expression vector pET30a ( + ) with multiple cloning sites. The whole sequence of NS1 gene in PPV SD1 strain was amplified by using PCR technology and the positive recombinant plasmid was analyzed by sequencing and homology comparison. The prokaryotic expression recombinant plasmid PET30a/NS1 was constructed to make its induction expression in Escherichia coll. [ Result] The target fragment with the length of 2 208 bp was obtained from PCR amplification. The nucleotide homologies between the cloned NS1 gene and the reported relevant PPV genes were from 97.3 % to 99.4 %, which indicated that NS1 gene had high conservation. But it had a 12-basepair successive deletion near the hydroxyl end. The cloned PPV NS1 gene was successfully expressed in prokaryotic cell, and its expression products existed mostly in inclusion bodies. [ Conclusion] The results of SDS-PAGE detection showed that the molecular weight of PPV NS1 protein was 86 KD. 展开更多
关键词 Porcine parvovirus NS1 gene cloning prokaryotic expression
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Cloning, Analysis and Prokaryotic Expression of DsSP Gene from Dunaliella salina
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作者 刘世才 柴晓杰 +2 位作者 郭卫华 王逸云 韩冬梅 《Agricultural Science & Technology》 CAS 2014年第6期907-915,共9页
[Objective] The purpose of this study was to clone a starch phosphorylase gene from Dunaliella salina and to preliminarily analyze its basic properties and protein expression. [Method] RT-PCR and RACE (rapid amplific... [Objective] The purpose of this study was to clone a starch phosphorylase gene from Dunaliella salina and to preliminarily analyze its basic properties and protein expression. [Method] RT-PCR and RACE (rapid amplification of cDNA ends) method was used for gene cloning; basic properties of the gene were analyzed using bioinformatics method; prokaryotic expression vector PGS21a-DsSP was constructed and transformed into E. coil BL21; the fusion protein was purified and detected by GST-SefinoseTM Kit and Western Blot, respectively. [Result] A starch phos-phorylase gene (GenBank accession No. KF061044) named DsSP was successfully isolated from D. salina. Basic properties, subcellular localization, secondary structure and tertiary structure of the protein were analyzed and predicted. The fusion protein was found in the supernatant and inclusion bodies. The supernatant protein was successfully purified. Western Blot analysis showed that the fusion protein was successfully expressed in E. coil BL21. [Conclusion] This study laid experimental foun- dation for further clarifying the function and mechanism of DsSP. 展开更多
关键词 Dunafiella salina Starch phosphorylase gene CLONE BIOINFORMATICS prokaryotic expression
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Gene cloning and prokaryotic expression of recombinant flagellin A from Vibrio parahaemolyticus 被引量:2
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作者 袁野 王秀利 +3 位作者 郭设平 刘洋 葛辉 仇雪梅 《Chinese Journal of Oceanology and Limnology》 SCIE CAS CSCD 2010年第6期1254-1260,共7页
The Gram-negative Vibrio parahaemolyticus is a common pathogen in humans and marine animals. Bacteria flagellins play an important role during infection and induction of the host immune response. Thus, flagellin prote... The Gram-negative Vibrio parahaemolyticus is a common pathogen in humans and marine animals. Bacteria flagellins play an important role during infection and induction of the host immune response. Thus, flagellin proteins are an ideal target for vaccines. We amplified the complete flagellin subunit gene (tTaA) from V. parahaemolyticus ATCC 17802. We then cloned and expressed the gene into Escherichia coli BL21 (DE3) cells. The gene coded for a protein that was 62.78 kDa. We purified and characterized the protein using Ni-NTA affinity chromatography and Anti-His antibody Western blotting, respectively. Our results provide a basis for further studies into the utility of the FlaA protein as a vaccine candidate against infection by Vibrio parahaemolyticus. In addition, the purified FlaA protein can he used for further functional and structural studies. 展开更多
关键词 Vibrio parahaemolyticus flagellin subunit gene (flail) cloning prokaryotic expression characterization
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Cloning, Expression of apxl Gene of Actinobacillus pleuropneumoniae and Development of ELISA 被引量:1
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作者 LIU Jian-jie, HE Qi-gai, CHEN Huan-chun, WU Bin, XU Xiao-juan, LIU Jun-fa, TANG Xian-chun and BEI Wei-chengCollege of Veterinary Medicine, Huazhong Agricultural University, Wuhan 430070 , P.R. China 《Agricultural Sciences in China》 CAS CSCD 2003年第5期578-582,共5页
Based on the published nucleotide sequence of the apxICA of Actinobacillus pleuropneumoniae in Genbank(S4074), a pair of primers were designed. A 3 640 bp(4 687 - 8 326 bp)gene fragment was amplified by PCR from the i... Based on the published nucleotide sequence of the apxICA of Actinobacillus pleuropneumoniae in Genbank(S4074), a pair of primers were designed. A 3 640 bp(4 687 - 8 326 bp)gene fragment was amplified by PCR from the isolated strain of A. pleuropneumoniae serovar 1. Then, it was cloned into pMD18-T, identified by both restriction endonuclease and sequence analysis, and inserted into pET-28a expression vector to yield the expression plasmid. SDS-PAGE result indicated expression of apxICA in BL21 (DE3), Western blot analysis showed the protein's immunogenicity. Using the expressed protein, ELISA was established to detect serum antibody against ApxI. The feature of ELISA to detect highly virulent A. pleuropneumoniae strains infection was proved by primary clinical application. 展开更多
关键词 Actinobacillus pleuropneumoniae apxICA gene cloning prokaryotic expression ELISA
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Cloning, Sequence Analysis, and Prokaryotic Expression of the Porcine DECR1 Gene
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作者 Bugao Li Xiaohong Guo +3 位作者 Guoqing Cao Xiaofen Yang Xiaojing Wang Zhongxiao Zhou 《Journal of Animal Science and Biotechnology》 SCIE CAS 2011年第2期61-67,共7页
2,4-dienoyl-CoA reductase 1 ( DECR1 ) is the key rate-limiting enzyme in the metabolism of polyunsaturated fatty acids. Although this protein has been studied in a variety of mammals, its role in por- cine is yet to... 2,4-dienoyl-CoA reductase 1 ( DECR1 ) is the key rate-limiting enzyme in the metabolism of polyunsaturated fatty acids. Although this protein has been studied in a variety of mammals, its role in por- cine is yet to be fully elucidated. However, it is a candidate determinant/indicator of meat quality, growth traits, and carcass quality. Here, we employed RT-PCR and rapid amplification of cDNA ends (RACE) analysis to amplify the full-length cDNA of DECR1 from Mashen pig liver, and cloned it into the expression vector pET-32a+. After confirmation by sequencing and restriction analysis, the recombinant plasmid was transformed into E. coli BL21 cells. The cDNA of pig DECR1 contained 2,352 nucleotides, including a 987 bp open reading frame flanked by a 53 bp 5'-untranslated region (UTR) and a 1,312 bp 3'-UTR. The pig DECR1 coding sequence encoded 328 amino acid residues, which shared 99%, 88%, 87%, 87%, 87%, 87%, and 83% identity with those of Sus scrofa (predicted), Bos taurus, Homo sapiens, Macaca mulatta, Pan troglodytes, Equus caballus, Canis, and Mus musculus, respectively. SDS-PAGE analysis revealed that the recombinant protein was expressed and that the expression level reached its highest level after 4 h induction. Western blot analysis indicated that the molecular weight of the expressed protein was the same as that predicted, ap- proximately 35 kDa. Collectively these data provide the basis for further studies into the physiological functions and molecular mechanisms of the pig DE- CR1 gene. 展开更多
关键词 cloning DECR1 gene PIG prokaryotic expression RACE sequence analysis
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Cloning and Prokaryotic Expression of Canine IL-2 Gene
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作者 FEI Dong-liang BI Cong-ming +1 位作者 SU Yu-gang BAI Ren 《Animal Husbandry and Feed Science》 CAS 2011年第1期30-32,共3页
[ Objective] To clone and express canine IL-2 gene and thus to provide theoretical support for the development of novel immune enhancers and genetic engineering vaccines. [ Method] Leukocytes separated from canine who... [ Objective] To clone and express canine IL-2 gene and thus to provide theoretical support for the development of novel immune enhancers and genetic engineering vaccines. [ Method] Leukocytes separated from canine whole blood were stimulated by concanavalin for 20 h, and then total RNA was extracted. According to the sequence of canine IL-2 gene published in the GenBank, a pair of primers was designed. After PCR am- plificetion, the target fragment was cloned into prokaryotic expression vector pET-28a. The recombinants were transformed into the host bacteria BL21. After IPTG induction, the expression products were analyzed by SDS-PAGE. [ Result] A 500 bp band with the expected size appeared in the RT-PCR products. After the pMD18-T-IL2 was identified by double digestion, an approximately 500 bp fragment was produced, which indicated successful cloning of the gene. After the pET-28a-lL2 was identified by restriction enzyme digestion and PCR, a 500 bp fragment was produced, which indicated successful construction of the expression vector. As revealed by the SDS-PAGE analysis, a protein band with molecular weight of about 20 kDa appeared. [ Conclusion] The canine IL-2 gene was cloned and expressed. 展开更多
关键词 CANINE INTERLEUKIN-2 gene cloning prokaryotic expression
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cDNA Cloning, Prokaryotic Expression of Two Splicing Products of mLRG, a Mouse Gene of Lipopolysaccharide Response
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作者 Zhongming Dai Zanguo Nie +2 位作者 Liang He Lina Guan Yunsheng Yang 《International Journal of Clinical Medicine》 2015年第11期867-875,共9页
Aim: To clone two splicing products of the mouse mLRG-cDNA and to express mLRG protein. Methods: The sequence obtained was compared human lrg to mouse genome with a comparative BLAST genome search and found completely... Aim: To clone two splicing products of the mouse mLRG-cDNA and to express mLRG protein. Methods: The sequence obtained was compared human lrg to mouse genome with a comparative BLAST genome search and found completely identical. We spliced some fragments to a whole mouse lrg-cDNA sequence and designed a pair of primers at completely homologous fragments in 5’-UTR and 3’-UTR, we amplified mouse lrg-cDNA by RT-PCR. Then the sequence encoding the mLRG protein was amplified by RT-PCR from the total RNA of NIH3T3 cell stimulated by lps (lipopolysaccharide), and we got two splicing products of mLRG (mLRGW, mLRGS) and two sequences encoding protein were cloned into the prokaryotic expression vector pTAT so as to construct the recombinant expression vector pTAT-MLRGW and pTAT-MLRGS. The proteins were expressed in E. coli BL21 (DE3). Results: We got a cDNA fragment with the length of 1905 bp. Its location is at chromosome X qF4 site and we amplified two encoding regions covered 1554 bp and 1404 bp respectively (mlrgW mlrgS). His-TAT-mLRGW and His-TAT-mLRGS fusion protein were expressed successfully. mlrgW is consist of 10 exons and 9 introns;mlrgS is consist of 11exons and 10 introns. Conclusion: Cloning of two splicing products of mouse novel gene MLRG and prokaryotic protein expressions are of help in the further study of this gene. 展开更多
关键词 mLRG LIPOPOLYSACCHARIDE RESPONSE gene cDNA cloning prokaryotic Protein expression
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Cloning and Expression of Conserved Sequences of cry Gene in E.coli Strain Rosetta(DE3) 被引量:1
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作者 罗翠平 李金华 +1 位作者 谢烨明 曾万勇 《Agricultural Science & Technology》 CAS 2012年第5期958-961,996,共5页
[Objective] The aim was to clone the conserved sequences of cry gene and express them in Rosetta (DE3). [Method] Specific primers were designed according to NCBI database information and the conserved sequences of c... [Objective] The aim was to clone the conserved sequences of cry gene and express them in Rosetta (DE3). [Method] Specific primers were designed according to NCBI database information and the conserved sequences of cry gene were amplified by PCR from Bt transgenic cotton. Then recombinant plasmids were constructed and expressed in E. coil strain Rosetta (DE3). Finally, the effects of different concentrations and inducing time of IPTG on the expression level of protein were investigated. [Result] Two conserved sequences (304 and 853 bp respectively) of cry gene were amplified. The result of SDS-PAGE confirmed that the recombinant plasmids pGEX-4t-I-304 and pGEX-4t-1-853 could express fusion proteins by IPTG induction and the molecular weight of protein products was 39 and 62.4 kDa respectively, which was in accordance with predicted result. The optimal protein ex- pression conditions were confirmed as induction with 0.15 mmol/L IPTG for 7 h. [Conclusion] This study prepared the ground for the further detection of Bt transgenic crops. 展开更多
关键词 Bt gene Conserved sequence cloning prokaryotic expression
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Cloning and Expression of Wheat Heat-shock Protein 60 (HSP60) Gene in E.coli 被引量:1
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作者 李芳芳 王媛媛 +1 位作者 刘国富 曹雪松 《Agricultural Science & Technology》 CAS 2010年第1期5-7,共3页
[Objective]The aim was to construct the wheat heat-shock protein 60 (HSP60) gene in prokaryotic expression vector and express HSP60 efficiently in E.coli. [Method]According to the wheat HSP60 gene sequence in GenBan... [Objective]The aim was to construct the wheat heat-shock protein 60 (HSP60) gene in prokaryotic expression vector and express HSP60 efficiently in E.coli. [Method]According to the wheat HSP60 gene sequence in GenBank,a pair of primers P1/P2 were designed and synthesized. The wheat HSP60 gene fragment was amplified from the wheat RNA by RT-PCR and inserted into bacterial expression vector of pGEX-4T-1. The construct of pGEX-4T-1-HSP60 was subsequently transformed into E.coli BL21. [Result]The construct of pGEX-4T-1-HSP60 was verified by restriction endonuclease digestion and sequenced. Compared with the sequences of wheat HSP60 genes in GenBank,homology accounted to 100%. Expression of the GST-HSP60 fusion protein was induced with IPTG. Its molecular weight was about 90 kD. The result was identified by electrophoresis of SDS-PAGE. Expression of the protein bands was consistent with the expected size. [Conclusion]The recombinant prokaryotic expression vector in pGEX-4T-1-HSP60 was constructed successfully and expressed stably in E.coli BL21. This will lay the foundation for further study on the functions of the protein and its mechanism. 展开更多
关键词 HSP60 gene cloning prokaryotic expression
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Construction of recombinant plasmid and prokaryotic expression in E. Coli and biological activity analysis of human placenta arresten gene 被引量:7
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作者 Jin-Ping Zheng, Hai-Ying Tang, Xian-Jiu Chen, Bao-Feng Yu, Jun Xie and Tang-Chun Wu Department of Toxicology (and Department of Biochemistry and Molecular Biology Shanxi Medical University, Taiyuan 030001, China: Institute of Occupational Medicine, Tongji Medical College, Huazhong University of Science and Technology, Wuhan 430030, China 《Hepatobiliary & Pancreatic Diseases International》 SCIE CAS 2006年第1期74-79,共6页
BACKGROUND: The proliferation and metastasis of cancers depend on angiogenesis. This property provides the feasibility for the treatment of cancer by inhibition of angiogenesis, and many angiogenic inhibitors have bee... BACKGROUND: The proliferation and metastasis of cancers depend on angiogenesis. This property provides the feasibility for the treatment of cancer by inhibition of angiogenesis, and many angiogenic inhibitors have been demonstrated to effectively inhibit angiogenesis and consequently the growth of solid cancer. As for the newly identified angiogenesis inhibitor, arresten, some studies have found its high activity on restrainting tumor vessel. This study was to assess the anti-angiogenic activity of arresten. METHODS: The arresten gene was obtained from a healthy puerpera's placenta tissue by the reverse transcriptase-polymerase chain reaction (RT-PCR) method, and molecular cloning to prokaryotic expression plasmid pBV220 by recombination strategy. The prokaryotic expression plasmid pBV220/arr was identified by restriction enzyme digestion and sequenced. The pBV220/arr was transformed into E. coli JM109, DH5α, BL21 and BL21 (DE3) by the CaCl_2 transformation method. The arresten expression level was detected by SDS-PAGE. The expressed product was purlfled, re-naturalized and detected for its biological activity of inhibiting the angiogenesis of chorioallantoic membrane (CAM). RESULTS: The arresten gene was cloned and pBV220/arr was constructed. The arresten expression level of protein was highly increased after pBV220/arr was transformed into E. coli BL21 (DE3). SDS-PAGE showed that the expressed arresten proteins were mainly inclusion bodies and had a molecular weight of 26 kDa. The expressed arresten protein showed evident biological activities. CONCLUSIONS: The successful construction of recombinant plasmid pBV220/arr and the effective expression in E. coil have laid a foundation for further study of its anti-angiogenic function and may pave the way for future antitumor application. 展开更多
关键词 ARRESTEN prokaryotic expression vector gene cloning and expression biological activity
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Gene Cloning and Expression Analysis of G Protein αq Subunit from Helicoverpa assulta (Guenée) 被引量:3
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作者 QIAO Qi LI Hai-chao YUAN Guo-hui GUO Xian-ru LUO Mei-hao 《Agricultural Sciences in China》 CAS CSCD 2008年第2期187-192,共6页
The cDNA encoding the G protein αq subunit was isolated from the antennae of Helicoverpa assulta (Guen6e) by reverse transcription polymerase chain reaction (RT-PCR) and named as HassGαq. Sequencing analysis sho... The cDNA encoding the G protein αq subunit was isolated from the antennae of Helicoverpa assulta (Guen6e) by reverse transcription polymerase chain reaction (RT-PCR) and named as HassGαq. Sequencing analysis showed that the fulllength of HassGαq open reading frame (ORF) is 1 062 bp, 353 amino acid residues are encoded. The predicted molecular weights (MW) and isoelectric point (PI) are 41.5 kD and 5.15, respectively. HassGαq gene was then constructed into expression vector pGEX-4T-2 for over expression in prokaryotic cells. The SDS-PAGE and Western blot analysis showed that induced by Isopropyl-β-D-Thiogalactoside (IPTG), the GST-HassGαq fusion protein is expressed in Escherichia coil BL21, and its MW was found to be about 66 kD nearly equal to the predicted. In addition, RT-PCR analysis showed that the expressions of HassGαq are not tissue specific. 展开更多
关键词 Helicoverpa assulta G protein α subunit gene cloning prokaryotic expression expression pattern
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Vitis amuerensis CBF3 Gene Isolation,Sequence Analysis and Expression 被引量:5
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作者 WANG Zhan-bin FENG Lian-rong +1 位作者 WANG Jin-jie WANG Zhi-ying 《Agricultural Sciences in China》 CSCD 2010年第8期1127-1132,共6页
The full length cDNA sequence of CBF3 (CRT/DRE-binding factor) was cloned from Vitis amurensis by reverse transcription polymerase chain reaction (RT-PCR) using the primers designed based on CBF genes available in... The full length cDNA sequence of CBF3 (CRT/DRE-binding factor) was cloned from Vitis amurensis by reverse transcription polymerase chain reaction (RT-PCR) using the primers designed based on CBF genes available in GenBank. Sequence analysis showed that the gene had 854 bp long and its coding sequence contained 720 bp, encoding a protein with 239 amino acids and an AP2 structural domain. The molecular mass of CBF3 was predicted to be 25.9 kDa and its theoretical isoelectric point was 7.02 and aliphatic index was 59.29. The average hydropathicity of the protein was -0.551. The tertiary structures of CBF3 were also analyzed. The prokaryotic expression vector pGEX-4T-CBF3 containing CBF3 gene was constructed and CBF3 fusion protein (52 kDa) was produced in Escherichia coli after induction with 1 mmol L-1 IPTG. Further studies are needed to evaluate its potential application for improving plant resistance to cold and other stress condition such as drought and salinity. 展开更多
关键词 Vitis amurensis CBF gene cloning sequence analysis expression in prokaryote
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Characterization and Expression of Outer Membrane Protein A I Gene of Aeromonas veronii
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作者 Wang Hai-juan Wang Li 《Journal of Northeast Agricultural University(English Edition)》 CAS 2015年第2期15-21,共7页
The outer membrane protein, ompA, ofAeromonas veronii has a role in the virulence of the organism and is a potential candidate for vaccine development. In this study, ompA I ofAeromonas veronii strain WA106 was cloned... The outer membrane protein, ompA, ofAeromonas veronii has a role in the virulence of the organism and is a potential candidate for vaccine development. In this study, ompA I ofAeromonas veronii strain WA106 was cloned and sequenced, then, it was expressed in Escherichia coli BL21. The nucleotide sequence of ompA I gene was 1 023 base pairs (GenBank Accession NO.KC748024), which showed 100% homology with that of A. veronii (NO.AB290200.1). This predicted protein was composed of 340 amino acid residues. Its molecular weight was 35.78 ku and isoelectric point was 5.18. The protein was a hydrophilic protein containing alpha helix and random coil with percentage of 35.0% and 49.7%, respectively. The tertiary structure, quaternary structure prediction showed that ompA I protein contained two peptide chains. SDS-PAGE showed that the actual value of the fusion protein was consistent with the expected result. It will facilitate further study of the role of ompA I protein. 展开更多
关键词 Aeromonas veronii ompA I gene cloning SEQUENCING prokaryotic expression
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陆地棉GhUGP1基因的克隆与表达分析
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作者 足木热木·吐尔逊 李晨宇 +5 位作者 陈明 于月华 李晓荣 杨洋 王勇攀 李波 《西北农业学报》 CAS CSCD 北大核心 2024年第11期2038-2047,共10页
为进一步了解UGPase在棉花中的作用,根据全基因组测序结果,筛选且克隆了在陆地棉纤维发育过程中的关键基因GhUGP1。利用生物信息学方法对其核苷酸和氨基酸序列进行分析,通过同源重组技术,将GhUGP1基因的编码序列构建到原核表达载体pMAL-... 为进一步了解UGPase在棉花中的作用,根据全基因组测序结果,筛选且克隆了在陆地棉纤维发育过程中的关键基因GhUGP1。利用生物信息学方法对其核苷酸和氨基酸序列进行分析,通过同源重组技术,将GhUGP1基因的编码序列构建到原核表达载体pMAL-C4x上,通过IPTG诱导蛋白表达来确定IPTG诱导蛋白的最佳条件,最后利用Western Blot鉴定重组蛋白。结果显示,GhUGP1(XP_040931642.1)全长序列6572 bp,编码区1404 bp,编码467个氨基酸,预测分子质量约为51.493 ku,等电点为5.86。氨基酸序列比对分析发现在陆地棉、亚洲棉、木槿等不同物种间UGP序列的相似率为90.63%。进化树分析结果显示GhUGP1蛋白与亚洲棉UGP蛋白亲缘关系最近,同源性最高并在一个分支上。亚细胞定位结果显示该蛋白为核膜共定位。蛋白诱导时由于IPTG浓度梯度结果差别不明显,选择IPTG终浓度为0.3 mmol/L,而温度梯度和时间梯度结果差异明显,确定最佳诱导温度为28℃,最佳诱导时间为6 h,蛋白溶解及纯化的温度和时间为28℃诱导6 h。Western Blot结果表明重组蛋白的大小正确,最终成功获得了大小为95.9 ku的pMAL-C4x-GhUGP1重组蛋白,为后期对GhUGP1功能深度解析提供帮助。 展开更多
关键词 陆地棉 GhUGP1基因 克隆 序列分析 原核表达
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红肉火龙果果糖激酶基因HpFRK1克隆、表达与酶学活性分析
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作者 解璞 晏霜 +1 位作者 王红林 郑乾明 《西北植物学报》 CAS CSCD 北大核心 2024年第10期1589-1596,共8页
【目的】克隆红肉火龙果果糖激酶基因,检测其表达和酶活性,解析其对果实发育可溶性糖积累的生理功能。【方法】从‘紫红龙’果肉克隆HpFRK1基因,进行生物信息学和亚细胞定位分析,利用qRT-PCR检测基因表达,通过大肠杆菌诱导表达获得重组... 【目的】克隆红肉火龙果果糖激酶基因,检测其表达和酶活性,解析其对果实发育可溶性糖积累的生理功能。【方法】从‘紫红龙’果肉克隆HpFRK1基因,进行生物信息学和亚细胞定位分析,利用qRT-PCR检测基因表达,通过大肠杆菌诱导表达获得重组蛋白并检测酶活性。【结果】HpFRK1的开放阅读框长度为993bp,编码330个氨基酸,具有磷酸果糖激酶B家族结构域。HpFRK1与甜菜BvFRK亲缘关系最近,均属于细胞质定位的FRKs。HpFRK1在成熟茎和不同发育时期果实均表达,在花后20d的果实表达量最高,随果实发育逐渐下调,花后30d(果实成熟)表达量最低。亚细胞定位检测表明HpFRK1主要定位于细胞核和细胞质。诱导获得的Hp-FRK1重组蛋白特异性催化果糖磷酸化(Km为11.01mmol/L)。【结论】HpFRK1在细胞质特异性催化果糖磷酸化,在红肉火龙果果实发育期间负调控果实可溶性糖积累。 展开更多
关键词 红肉火龙果 果糖激酶 基因克隆 表达分析 原核表达
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牦牛FABP3基因克隆及组织表达谱分析 被引量:1
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作者 戴荣凤 黄纯 +3 位作者 扎老 路建卫 唐月琴 梁春年 《西北农林科技大学学报(自然科学版)》 CSCD 北大核心 2024年第1期1-8,共8页
【目的】分析牦牛心肌脂肪酸结合蛋白3(FABP3)基因的结构和功能,并检测其在成年牦牛和胎牛中的表达水平,为探究该基因在牦牛育种中的生物学功能提供理论参考。【方法】以美仁牦牛的心脏组织为试验材料,PCR扩增FABP3基因,对得到的编码区... 【目的】分析牦牛心肌脂肪酸结合蛋白3(FABP3)基因的结构和功能,并检测其在成年牦牛和胎牛中的表达水平,为探究该基因在牦牛育种中的生物学功能提供理论参考。【方法】以美仁牦牛的心脏组织为试验材料,PCR扩增FABP3基因,对得到的编码区序列(CDS)进行生物信息学分析;利用实时荧光定量PCR(RT-qPCR),检测FABP3基因在成年牦牛和胎牛心脏、肝脏、脾脏、肺脏、肾脏及肌肉组织的表达水平。【结果】牦牛FABP3基因编码区序列长度为402 bp,编码133个氨基酸;蛋白质的高级结构主要是β-转角和延伸链;牦牛FABP3蛋白不存在跨膜区域和信号肽,属于具有一定亲水性的稳定蛋白;牦牛FABP3基因CDS区核苷酸及其编码氨基酸序列的同源性分析显示,FABP3基因在牛属动物中具有一定的保守性;系统进化树分析表明,牦牛与野牦牛和瘤牛的亲缘关系最近,与鸡的亲缘关系最远。RT-qPCR结果显示,FABP3基因在成年牦牛和胎牛的心脏、肝脏、脾脏、肺脏、肾脏及肌肉组织中均有表达,但在胎牛肝脏、脾脏、肾脏和肌肉中的表达水平显著或极显著高于成年牦牛,在成年牦牛肺脏中的表达水平极显著高于胎牛。【结论】克隆了牦牛FABP3基因,探究了FABP3基因在牦牛中的组织表达规律,为进一步研究该基因在牦牛脂肪沉积中的作用提供了基础数据。 展开更多
关键词 美仁牦牛 FABP3 基因克隆 生物信息学 组织表达谱
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河虾过敏原原肌球蛋白的基因克隆与原核表达
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作者 骆叶晴 郑双艳 +4 位作者 孙耀斌 陈娇 刘鑫 陈红兵 谢彦海 《食品科学》 EI CAS CSCD 北大核心 2024年第13期89-95,共7页
为了探寻天然原肌球蛋白的可替代物作为诊断和治疗虾类过敏的基础材料,本研究从河虾中提取总RNA,利用cDNA末端快速扩增技术克隆河虾过敏原原肌球蛋白基因的全长序列。以此序列设计表达引物,构建表达载体,最后通过异丙基-β-D-硫代半乳糖... 为了探寻天然原肌球蛋白的可替代物作为诊断和治疗虾类过敏的基础材料,本研究从河虾中提取总RNA,利用cDNA末端快速扩增技术克隆河虾过敏原原肌球蛋白基因的全长序列。以此序列设计表达引物,构建表达载体,最后通过异丙基-β-D-硫代半乳糖苷(isopropyl-β-D-thiogalactopyranoside,IPTG)诱导表达重组原肌球蛋白。结果显示,河虾的原肌球蛋白基因cDNA序列全长1658 bp,开放阅读框855 bp,编码284个氨基酸,预测蛋白等电点4.70,预测分子质量32.8 kDa。河虾原肌球蛋白cDNA序列已上传至GenBank数据库,登录号为OP974621。本研究成功构建河虾原肌球蛋白重组表达质粒pET-30a-TM,并用IPTG进行体外诱导表达,最佳诱导条件为IPTG浓度1 mmol/L、37℃诱导4 h。可溶性分析结果表明重组原肌球蛋白主要以可溶性形式存在于细胞破碎液的上清液中,分子质量约38 kDa。 展开更多
关键词 河虾 原肌球蛋白 基因克隆 原核表达 重组蛋白
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灰毡毛忍冬花器官发育相关LmSOC1基因克隆及表达分析
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作者 龙丽君 马英姿 +4 位作者 曾慧杰 李昌珠 张岗 刘思思 李依民 《中南林业科技大学学报》 CAS CSCD 北大核心 2024年第5期181-190,共10页
【目的】克隆灰毡毛忍冬MADS-box家族基因SOC1(SUPPRESSOR OF OVEREXPRESSION OF CO1),对其进行生物信息学和表达模式分析,为探究灰毡毛忍冬花冠不开放机制奠定理论基础。【方法】基于花蕾型灰毡毛忍冬转录组数据,筛选到开花调控基因LmS... 【目的】克隆灰毡毛忍冬MADS-box家族基因SOC1(SUPPRESSOR OF OVEREXPRESSION OF CO1),对其进行生物信息学和表达模式分析,为探究灰毡毛忍冬花冠不开放机制奠定理论基础。【方法】基于花蕾型灰毡毛忍冬转录组数据,筛选到开花调控基因LmSOC1的Unigene序列并克隆全长cDNA序列,通过生物信息学分析和实时荧光定量PCR技术分析编码蛋白特性和不同品种中LmSOC1基因的表达特异性,最后将LmSOC1基因插入到原核表达质粒载体pTOPO-D1中,并在表达宿主BL21(DE3)中进行蛋白表达。【结果】LmSOC1基因包含645bp的ORF区,LmSOC1蛋白不含信号肽、无跨膜区,为稳定的亲水性蛋白。系统进化树分析表明,LmSOC1蛋白与黄花蒿、榴莲、可可等的SOC1蛋白亲缘关系更近。实时荧光定量PCR分析表明,在2个花蕾型灰毡毛忍冬品种的花蕾和叶片中均检测到LmSOC1基因的表达,而叶片中表达量明显高于花蕾。同时,在早期花蕾中LmSOC1基因的表达量高于晚期花蕾,在‘金翠蕾’品种中这一表达差异极显著(P<0.01)。最后成功在大肠杆菌BL21(DE3)中表达出重组蛋白。【结论】通过对LmSOC1基因的克隆和表达分析发现,该基因可能在灰毡毛忍冬花器官发育过程中发挥重要作用,为进一步研究该基因在植物花发育中的生物学功能奠定了基础。 展开更多
关键词 灰毡毛忍冬 MADS-BOX LmSOC1 基因克隆 表达分析 原核表达
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美仁牦牛MYL 9基因克隆、生物信息学分析及组织表达研究
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作者 马荣 喇永福 +6 位作者 包鹏甲 郭宪 路建卫 扎老 赵雪 梁春年 成述儒 《中国畜牧兽医》 CAS CSCD 北大核心 2024年第4期1410-1419,共10页
【目的】克隆美仁牦牛肌球蛋白轻链9(myosin light chain 9,MYL9)基因CDS区并对其进行生物信息学分析,检测MYL 9基因的组织表达特征,为探究该基因功能提供一定理论依据。【方法】以美仁牦牛肌肉组织cDNA为模板,利用PCR扩增并克隆美仁牦... 【目的】克隆美仁牦牛肌球蛋白轻链9(myosin light chain 9,MYL9)基因CDS区并对其进行生物信息学分析,检测MYL 9基因的组织表达特征,为探究该基因功能提供一定理论依据。【方法】以美仁牦牛肌肉组织cDNA为模板,利用PCR扩增并克隆美仁牦牛CDS区序列,与其他物种进行相似性比对及系统进化树构建;通过在线软件对MYL9蛋白进行生物信息学分析,利用实时荧光定量PCR检测MYL 9基因在美仁牦牛心脏、肝脏、脾脏、肺脏、肾脏、肌肉、脂肪和睾丸组织中表达情况。【结果】美仁牦牛MYL 9基因CDS区长516 bp,共编码171个氨基酸。系统进化树结果显示,美仁牦牛与野牦牛、普通牛亲缘关系最近,与高山倭蛙亲缘关系最远。MYL9蛋白分子式为C 858 H 1324 N 234 O 274 S 12,原子数为2702,理论等电点为4.85,不稳定系数和总平均亲水性分别为37.22和―0.772,属于稳定亲水性蛋白。MYL9蛋白无信号肽和跨膜螺旋结构,属于非分泌性蛋白;主要定位于线粒体、细胞核、细胞质中,具有17个特异性磷酸化位点。MYL9蛋白二级结构主要由α-螺旋、无规则卷曲、β-折叠和延伸链构成,三级结构预测结果与二级结构一致。实时荧光定量PCR结果显示,MYL 9基因在美仁牦牛心脏、肝脏、脾脏、肺脏、肾脏、肌肉、脂肪和睾丸组织中均表达,且肝脏和肌肉组织中表达量显著高于其他组织(P<0.05)。【结论】本研究成功克隆美仁牦牛MYL 9基因CDS区,探究了MYL 9基因的生物学功能及组织表达特征,研究结果为进一步探究牦牛MYL 9基因功能特征提供了参考。 展开更多
关键词 美仁牦牛 MYL 9基因 克隆 生物信息学 组织表达
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