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IDENTIFICATION OF PATHOGENIC LEPTOSPIRES BY RECOMBINANT DNA PROBES
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作者 戴保民 肖建国 沈成义 《Chinese Medical Sciences Journal》 CAS CSCD 1994年第4期209-214,共6页
Early diagnosis of leptospirosis of pulmonary diffuse hernorrhage type (PDH) is of crucial importance in saving patients. To develop a sensitive and specific methed for diagnosis, a genomic library of the main pathoge... Early diagnosis of leptospirosis of pulmonary diffuse hernorrhage type (PDH) is of crucial importance in saving patients. To develop a sensitive and specific methed for diagnosis, a genomic library of the main pathogen of PDH, L. interrogans serovar lai strain 017, was constructed with the plasmid vector PUC9. Recombinant plasmids which have hornologous fragments of pathogenic leptospires were screened from the bank. A recombinant plasmid,designated PCX7, could detect 1.7 kb fragment of strain 017, 9. 0 kb of strain 601 and 30. 0 kb of strain Hebdomadis, respectively, without cross hybridization with nonpathogenic leptospires such as L. biflexa strain Patoc I and hoptonema illini. The recombinant plasmid PCX7 could detect pathogenic leptospires which are the main pathogens endemic to Sichuan Province. 展开更多
关键词 LEPTOSPIRA recombinant dna Southern hybridization
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Immunogenicity analysis following human immunodeficiency virus recombinant DNA and recombinant vaccinia virus Tian Tan prime-boost immunization 被引量:7
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作者 LIU CunXia DU ShouWen +9 位作者 LI Chang WANG YuHang WANG MaoPeng LI Yi YIN RongLan LI Xiao REN DaYong QIN YanQing REN JingQiang JIN NingYi 《Science China(Life Sciences)》 SCIE CAS 2013年第6期531-540,共10页
This study assessed and compared the immunogenicity of various immunization strategies in mice using combinations of re- combinant DNA (pCCMp24) and recombinant attenuated vaccinia virus Tian Tan (rddVTT_ccMpe4). ... This study assessed and compared the immunogenicity of various immunization strategies in mice using combinations of re- combinant DNA (pCCMp24) and recombinant attenuated vaccinia virus Tian Tan (rddVTT_ccMpe4). Intramuscular immuniza- tion was performed on days 0 (prime) and 21 (boost). The immunogenicity of the vaccine schedules was determined by meas- uring human immunodeficiency virus (HIV)-specific binding antibody levels and cytokine (interleukin-2 and interleukin-4) concentrations in peripheral blood, analyzing lymphocyte proliferation capacity against HIV epitopes and CD4~/CD8+cell ratio, and monitoring interferon-gamma levels at different times post-immunization. The results showed that pCCMp24, rddVTT.ccMp24 and their prime-boost immunization induced humoral and cellular immune responses. The pCCMp24/ rddVTT.ccMp24 immunization strategy increased CD8+ T cells and induced more IFN-7-secreting cells compared with sin- gle-shot rDNA. The prime-boost immunization strategy also induced the generation of cellular immunological memory to HIV epitope peptides. These results demonstrated that prime-boost immunization with rDNA and rddVTT_ccMp24 had a tendency to induce greater cellular immune response than single-shot vaccinations, especially IFN-7 response, providing a basis for further studies. 展开更多
关键词 vaccinia virus Tian Tan human immunodeficiency virus recombinant dna PRIME-BOOST IMMUNOGENICITY
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Construction of recombinant adeno-associated viral vectors in human neurenergen-3 gene 被引量:1
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作者 Xiangli Wang Haili Wang Baojie Mi 《Neural Regeneration Research》 SCIE CAS CSCD 2007年第6期335-338,共4页
BACKGROUND: Research of transgene brings hope for gene therapy of various diseases; in addition, some projects have been tested in clinic. Recently, the focus has been to find an ideal vehicle and a suitable therapeu... BACKGROUND: Research of transgene brings hope for gene therapy of various diseases; in addition, some projects have been tested in clinic. Recently, the focus has been to find an ideal vehicle and a suitable therapeutic gene. OBJECTIVE: To explore an effective way to construct recombinant adeno-associated viral vectors expression in human neurnnergen-3 gene. DESIGN: Gene directed cloning. SETTING: Central Laboratory of Northern China Coal Medical College. MATERIALS: DH5a competent bacillus coli strain was provided by Capital Medical University; pCDNA3-NT-3 by professor Chen from Bengbu Medical College; pAAV-Laze, pAAV-Helper, pAAV-RC and pAAV-MCS plasmids by Capital Medical University; HEK293 cells by Cell Center of Basic Medical College of Tongji Medical University. METHODS: NT-3 genes which were selected from pCDNA3-NT-3 plasmids were cloned in pAAV-MCS to form a recombinant adeno-associated viral plasmid (pAAV-NT-3). pAAV-NT-3, pAAV-RC, pAAV-LacZ and pHelper plasmids were extracted, purified and subjected to enzyme-shearing evaluation. In addition, pAAV-NT-3 and pAAV-LacZ were cotransfected with pHelper and pAAV-RC, respectively into AVV-293 cells with DNA mediated by calcium superphosphate transfection gene; and then, AVV-293 cells were packed into recombinant adeno-associated viral rAAV-NT-3 and rAAV-LacZ. After collection of viral particles, rAAV-LacZ viral stock solution was diluted based on ratio of 10:1 and the mixture was used to infect HT 1080 cells. X-gal stain was used to measure virus titer. MAIN OUTCOME MEASURES: Size of targeted gene fragments, validity of vehicle construction and virus titer. RESULTS: Targeted gene NT-3 was successfully inserted into the relative vehicle pAAV and pAAV-NT-3 was correctly recongnized by enzyme-shearing evaluation. Enzyme-shearing electrophoresis demonstrated that pAAV-NT-3, pAAV-RC, pAAV-LacZ and pHelper plasmids were successfully extracted and purified. β-galactoside staining in situ indicated that LacZ genes were expressed in human fibrosarcoma cells (HT1080) and the recombinant virus titer was measured as 1 ×10^12 virus particles per milliliter. CONCLUSION: Total-length cDNA fragment of NT-3 gene, which is obtained from pCDNA3-NT-3 plasmids, is closely matched to polyclone enzyme-shearing sites of adeno-associated viral vectors, while the combination can be used to construct recombinant adeno-associated viral vectors expression in hNT-3 gene. 展开更多
关键词 NEUROTROPHIN-3 cloning molecular adenoviruses human dna recombinant
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人c-fos原癌基因cDNA克隆及核酸序列分析 被引量:1
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作者 杨宝学 杨贵贞 《白求恩医科大学学报》 CSCD 1994年第2期106-108,共3页
本研究应用逆转录PCR方法从Jurkat传代细胞株获得一380bp的人c一fos原癌基因cDNA片段,并将其克隆到具有双向转录启动子的载体质粒pGEM3Zf(+)中。核酸序列分析表明,所克隆的cDNA片段包括人c-f... 本研究应用逆转录PCR方法从Jurkat传代细胞株获得一380bp的人c一fos原癌基因cDNA片段,并将其克隆到具有双向转录启动子的载体质粒pGEM3Zf(+)中。核酸序列分析表明,所克隆的cDNA片段包括人c-fos基因外显子2的大部分,外显子3的全部及外显子4的一部分。该重组质粒可分别用于制备c-foscDNA探针和RNA探针,为c-fos基因结构、表达调控等方面的研究奠定了工作基础。 展开更多
关键词 dna重组 分子克隆 癌基因
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Advances in Trehalose Biosynthesis Pathways and Application of Molecular Biology Technique 被引量:4
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作者 巩涛 李琳琳 +1 位作者 赵正中 刘德海 《Agricultural Science & Technology》 CAS 2016年第8期1790-1795,共6页
This paper aims to provide better guidance for construction of trehalose-producing recombinant strains to further improve the yield of trehalose. The research progress on trehalose biosynthesis pathways and the applic... This paper aims to provide better guidance for construction of trehalose-producing recombinant strains to further improve the yield of trehalose. The research progress on trehalose biosynthesis pathways and the application of molecular biology technique in trehalose study in recent 30 years, especially the last 10 years are reviewed. Results show that there are 5 pathways of trehalose synthesis. Although enzymes and genes of trehalose synthesis have been isolated and genetic engineering strains have increased gradually, the improvement of trehalose yield is still inadequate because most recombinant strains are limited to study the physicochemical properties of single enzyme. With the development of modern biological technology, especially the rapid development of DNA recombinant technology, metagenomics and synthetic biology, high expression of heterologous trehalose in recombinant strains would become a hot research topic in the future. 展开更多
关键词 TREHALOSE Biosynthesis pathway dna recombination technology METAGENOMICS
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Construction of a recombinant plasmid harbouring the rhoptry protein 1 gene of Toxoplasma gondii and preliminary observations on DNA immunity 被引量:2
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作者 陈观今 郭虹 +1 位作者 吕芳丽 郑焕钦 《Chinese Medical Journal》 SCIE CAS CSCD 2001年第8期54-57,107,共5页
Objective To observe the immune responses elicited in BALB/c mice by a DNA vaccine. A gene encoding rhoptry protein 1 (ROP1) from Toxoplasma gondii (T. gondii) was cloned into vector pcDNA3. Methods Amplifyied gene ... Objective To observe the immune responses elicited in BALB/c mice by a DNA vaccine. A gene encoding rhoptry protein 1 (ROP1) from Toxoplasma gondii (T. gondii) was cloned into vector pcDNA3. Methods Amplifyied gene fragments coding for ROP1 from the genomic DNA of T.gondii ZS2 were inserted into cloning vector, pUC18, and sub-cloned into pcDNA3. Mice were injected at a dosage of 100?μg recombinant plasmid DNA by intramuscular injection and boosted after 2 weeks. pcDNA3 and normal saline were used as control. 30, 50 and 70 days after the second immunization, NK cell activity, T lymphocyte proliferation and sub-clusters and serum IgG antibody were assayed.Results The specific gene fragment coding for ROP1 was amplified and a pcROP1 recombinant was constructed. At 30 days after immunization, the spleens of the mice were obviously enlarged evidently. NKC activity and the proliferation of spleen T lymphocytes seen on MTT assay were higher in pcROP1 group than in the controls. The number of CD4+ T cells exhibited no obvious increase compared with that of the control, but CD8+ T cells were obviously increased (P<0.05). At 90 days after vaccination, the titer of IgG antibody in the serum of vaccinated mice was positive (1∶100). Conclusion pcROP1 was constructed and it could elicit both cellular and humoral immune responses in immunized mice. 展开更多
关键词 Toxoplasma gondii · rhoptry protein 1 · pcROP1 recombinant plasmid · cloning · dna immunity
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GFAP promoter directs lacZ expression specifically in a rat hepatic stellate cell line 被引量:4
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作者 Gunter Maubach Michelle Chin Chia Lim 《World Journal of Gastroenterology》 SCIE CAS CSCD 2006年第5期723-730,共8页
AIM: The GFAP was traditionally considered to be a biomarker for neural gila (mainly astrocytes and nonmyelinating Schwann cells). Genetically, a 2.2-kb human GFAP promoter has been successfully used to target astr... AIM: The GFAP was traditionally considered to be a biomarker for neural gila (mainly astrocytes and nonmyelinating Schwann cells). Genetically, a 2.2-kb human GFAP promoter has been successfully used to target astrocytes in vitro and in vivo. More recently, GFAP was also established as one of the several makers for identifying hepatic stellate cells (HSC). In this project, possible application of the same 2.2-kb human GFAP promoter for targeting HSC was investigated. METHODS: The GFAP-lacZ transgene was transfected into various cell lines (HSC, hepatocyte, and other nonHSC cell types). The transgene expression specificity was determined by X-gal staining of the β-galactosidase activity. And the responsiveness of the transgene was tested with a typical pro-fibrotic cytokine TGF-β1. The expression of endogenous GFAP gene was assessed by real-time RT-PCR, providing a reference for the transgene expression. RESULTS: The results demonstrated for the first time that the 2.2 kb hGFAP promoter was not only capable of directing HSC-specific expression, but also responding to a known pro-fibrogenic cytokine TGF-β1 by upregulation in a doseand time-dependent manner, similar to the endogenous GFAP. CONCLUSION: In conclusion, these findings suggested novel utilities for using the GFAP promoter to specifically manipulate HSC for therapeutic purpose. 展开更多
关键词 Promoter Regions (Genetics) Animals Base Sequence Cell Line dna recombinant Gene Expression Glial Fibrillary Acidic Protein HEPATOCYTES Humans Lac Operon RNA Messenger Rats TRANSFECTION Transforming Growth Factor beta Transforming Growth Factor beta1
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Copper-Controllable, Site-Specific DMA Excision in Transgenic Plants
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作者 PENG Xiang-lei, LIANG Bin, CHEN Ming, HU Yuan-lei and LIN Zhong-ping(National Key Laboratory of Protein Engineering and Plant Genetic Engineering , Peking University , Beijing 100871 , P. R. China) 《Agricultural Sciences in China》 CAS CSCD 2003年第6期597-601,共5页
A copper-inducible, Cre-loxP recombination-mediated DNA excision system has been developed in transgenic tobacco plants. The copper inducible system derived from yeast was used for the control of the expression of the... A copper-inducible, Cre-loxP recombination-mediated DNA excision system has been developed in transgenic tobacco plants. The copper inducible system derived from yeast was used for the control of the expression of the Cre recombinase. Upon copper induction, the GVS reporter gene expression unit flanked by two direct lox sites was excised from the transgenic tobacco genome. Quantitative fluorometric GUS assays, Northern blot and PCR analyses showed a high-efficient, copper-dependent and Cre-loxP mediated DNA recombination in all the tested transgenic lines. The copper inducible foreign gene excision might be of great potential in genetic control of transgenic crops. 展开更多
关键词 Transgenic plants Copper-inducible system MRE CRE-LOXP dna recombination
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Construction of Eukaryotic Expression Vector pBlacz and Its Expression Both in Vitro and In Vivo
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作者 屈伸 杨仕林 +2 位作者 尤颖健 刘绍春 何善述 《Journal of Huazhong University of Science and Technology(Medical Sciences)》 SCIE CAS 1996年第1期14-17,共4页
A novel eukaryotic expression vector pBlacZ was constructed, which was transfected into the cell lines of NIH/3T3, COS-1, CHO and the primary culture of murine dermatic fibroblasts in vitro, and also into the murine s... A novel eukaryotic expression vector pBlacZ was constructed, which was transfected into the cell lines of NIH/3T3, COS-1, CHO and the primary culture of murine dermatic fibroblasts in vitro, and also into the murine subcutaneous layer and skeletal muscles of rats in vivo. It was detected that the gene expression vector could encode the E. Coli β-galactosidase effectively in all these histocytes. The results suggested that pBlacZ, as a novel expression vector, might have certain value of application. 展开更多
关键词 dna recombination gene transfer gene expression Β-GALACTOSIDASE
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不用接头进行异末端DNA重组的方法
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作者 谭德勇 邓双胜 《云南大学学报(自然科学版)》 CAS CSCD 1996年第2期103-105,108,共4页
用过渡载体通过两次重组进行不同粘性末端之间的DNA重组.该方法不需要替换接头,从而省去昂贵的试剂和平末端连接这种较难的操作,既经济,简单又有效,易于操作.
关键词 异末端连接 dna重组 过渡载体 重组
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Molecular evolutionary analysis of gene families encoding DNA recombination and repair proteins and histone demethylases,and their functional implications
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作者 马红 《生物物理学报》 CAS CSCD 北大核心 2009年第S1期5-5,共1页
Many eukaryotic genes are members of multi-gene families due to gene duplications, which generate new copies that allow functional divergence. However, the relationship between
关键词 GENE Molecular evolutionary analysis of gene families encoding dna recombination and repair proteins and histone demethylases and their functional implications dna
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Applications of 3D printed chimeric DNA biomaterials
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作者 Stephanie Dobres Giridhar Mula +1 位作者 Jonathan Sauer Donghui Zhu 《Engineered Regeneration》 2022年第1期13-23,共11页
The influence of genetic engineering on daily life is prominent,from genetically modified food to transgenic,antibiotic resistant plants.The direct manipulation of an organism’s genotype has opened the door to a myri... The influence of genetic engineering on daily life is prominent,from genetically modified food to transgenic,antibiotic resistant plants.The direct manipulation of an organism’s genotype has opened the door to a myriad of applications in an effort to treat chronic diseases.This paper proposes the unification of chimeric DNA technology and three-dimensional bioprinting to spark the development of new therapies.While studies of chimeric DNA,i.e.recombinant DNA,have been conducted since 1970,bioprinting is a budding method for tissue engineering and regenerative medicine.Both technologies are further described in the background section of this paper,and followed by a detailed analysis into current research,benefits,and limitations of 3D printed chimeric biomate-rials.Major benefits include low-cost and effective treatments for cancer,bio-morphological nanostructures for targeted drug delivery,personalized medicine with the use of stem cells,and a significantly reduced rate of addi-tional surgeries and transplant rejection after implantation.However,there are several shortcomings with current chimeric DNA applications,e.g.CAR-T cell therapies,and ethical dilemmas regarding the creation and regulation of human-animal chimeras.This review then presents future directions,in which inks made from chimeric DNA and live cells can be printed into bioactive engineered tissue,or biodegradable vehicles for targeted delivery of hiPSCs or CAR T-cells.Finally,this review concludes with a reaffirmation of its main points and the authors’thoughts on the potential of 3D printed chimeric biomaterials. 展开更多
关键词 Chimeric dna biomaterials Chimeric biomaterials recombinant dna 3D printing BIOPRINTING Tissue engineering Regenerative medicine CAR T-cell therapy
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DNA End Resection:Facts and Mechanisms 被引量:2
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作者 Ting Liu Jun Huang 《Genomics, Proteomics & Bioinformatics》 SCIE CAS CSCD 2016年第3期126-130,共5页
DNA double-strand breaks(DSBs),which arise following exposure to a number of endogenous and exogenous agents,can be repaired by either the homologous recombination(HR)or non-homologous end-joining(NHEJ) pathways... DNA double-strand breaks(DSBs),which arise following exposure to a number of endogenous and exogenous agents,can be repaired by either the homologous recombination(HR)or non-homologous end-joining(NHEJ) pathways in eukaryotic cells.A vital step in HR repair is DNA end resection,which generates a long 30single-stranded DNA(ss DNA) tail that can invade the homologous DNA strand.The generation of 30 ss DNA is not only essential for HR repair,but also promotes activation of the ataxia telangiectasia and Rad3-related protein(ATR).Multiple factors,including the MRN/X complex,C-terminal-binding protein interacting protein(Ct IP)/Sae2,exonuclease 1(EXO1),Bloom syndrome protein(BLM)/Sgs1,DNA2 nuclease/helicase,and several chromatin remodelers,cooperate to complete the process of end resection.Here we review the basic machinery involved in DNA end resection in eukaryotic cells. 展开更多
关键词 dna end resection Homologous recombination dna double-strand breaks Chromatin remodeling factors Genome stability
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Assembly of long DNA sequences using a new synthetic Escherichia coli-yeast shuttle vector 被引量:3
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作者 Zheng Hou Zheng Zhou +1 位作者 Zonglin Wang Gengfu Xiao 《Virologica Sinica》 SCIE CAS CSCD 2016年第2期160-167,共8页
Synthetic biology is a newly developed field of research focused on designing and rebuilding novel biomolecular components, circuits, and networks. Synthetic biology can also help understand biological principles and ... Synthetic biology is a newly developed field of research focused on designing and rebuilding novel biomolecular components, circuits, and networks. Synthetic biology can also help understand biological principles and engineer complex artificial metabolic systems. DNA manipulation on a large genome-wide scale is an inevitable challenge, but a necessary tool for synthetic biology. To improve the methods used for the synthesis of long DNA fragments, here we constructed a novel shuttle vector named p GF(plasmid Genome Fast) for DNA assembly in vivo. The BAC plasmid p CC1 BAC, which can accommodate large DNA molecules, was chosen as the backbone. The sequence of the yeast artificial chromosome(YAC) regulatory element CEN6-ARS4 was synthesized and inserted into the plasmid to enable it to replicate in yeast. The selection sequence HIS3, obtained by polymerase chain reaction(PCR) from the plasmid p BS313, was inserted for screening. This new synthetic shuttle vector can mediate the transformation-associated recombination(TAR) assembly of large DNA fragments in yeast, and the assembled products can be transformed into Escherichia coli for further amplification. We also conducted in vivo DNA assembly using p GF and yeast homologous recombination and constructed a 31-kb long DNA sequence from the cyanophage PP genome. Our findings show that this novel shuttle vector would be a useful tool for efficient genome-scale DNA reconstruction. 展开更多
关键词 yeast plasmid shuttle dna recombination Genome assembly inserted amplification homologous
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A novel treatment for weight reduction by the recombinant "Pichia pastoris" yeast expressing the hybrid protein of "irisin-furin-transferrin"
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作者 Mahsa Jalili Zahra Bazi Azita Hekmatdoost 《Journal of Integrative Medicine》 SCIE CAS CSCD 2016年第1期1-4,共4页
Obesity is a major health problem across the world, but there are few ways to effectively treat or manage it in the long term. Researchers are searching for more convenient, cost-effective and noninvasive therapies fo... Obesity is a major health problem across the world, but there are few ways to effectively treat or manage it in the long term. Researchers are searching for more convenient, cost-effective and noninvasive therapies for overweight and obese people. Recent studies have illustrated that the microbiome of the body's different organs can be used as a vehicle for in-situ gene therapy. We suggest that the recombinant form of "Pichia pastoris" yeast expressing the hybrid protein of "irisin-furin-transferrin" under the control of the enolase 1 promoter is a new nutraceutical strategy to absorb fewer calories from intestinal nutrients, and induce a higher metabolic rate to expend more calories, similar to that from engaging in physical activity. By comparison, this method can be a long-term, noninvasive treatment and can be used for obese patients who have movement limitations. 展开更多
关键词 obesity nutrition BIOTECHNOLOGY dna recombinant
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Multi-functions of exonuclease 1 in DNA damage response and cancer susceptibility
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作者 Shuang Yan Shanshan Gao Pingkun Zhou 《Radiation Medicine and Protection》 2021年第4期146-154,共9页
Exonuclease 1(EXO1)can catalyze nucleotide chain excision with its conserved N-terminal domain of 5′ to 3′ exonuclease activity,enabling it to influence diverse biological processes facing the challenges of genotoxi... Exonuclease 1(EXO1)can catalyze nucleotide chain excision with its conserved N-terminal domain of 5′ to 3′ exonuclease activity,enabling it to influence diverse biological processes facing the challenges of genotoxic environmental factors such as ionizing radiation.This nuclease activity enables EXO1 to maintain replication forks and telomeres length,to facilitate post-replication DNA repair and to process the end resection step of homologous recombination of DNA double-strand breaks-induced by ionizing radiation.When DNA replication is disrupted or blocked,EXO1 can cleave the broken DNA ends to form 3’ssDNA,leading to repair pathways activation.Excess EXO1-mediated nucleotide excision,however,can introduce an abundance of single-stranded DNA that can cause mutation and recombination via micro-homology-mediated end joining or single-strand annealing mechanisms,contributing to a loss of genetic information.EXO1 activity must therefore be carefully regulated within healthy cells.The mutations and dysregulations of EXO1 can increase the sensitivity of cells to radiation injury and risk of oncogenic transformation,limit the adoption of specific treatments in a range of human diseases.As such,EXO1 represents a promising target for the treatment and prevention of cancer.In the present review,we delineate the structural properties and functional characteristics of EXO1,discuss the relationship between this exonuclease and cancer susceptibility as well as the second cancers related to radiotherapy. 展开更多
关键词 Exonuclease 1(EXO1) RADIOTHERAPY dna double-strand break(DSB) dna recombination Cancer susceptibility dna end resection
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The archaeal KEOPS complex possesses a functional Gon7 homolog and has an essential function independent of the cellular t^(6)A modification level
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作者 Pengju Wu Qi Gan +6 位作者 Xuemei Zhang Yunfeng Yang Yuanxi Xiao Qunxin She Jinfeng Ni Qihong Huang Yulong Shen 《mLife》 CSCD 2023年第1期11-27,共17页
Kinase,putative Endopeptidase,and Other Proteins of Small size(KEOPS)is a multisubunit protein complex conserved in eukaryotes and archaea.It is composed of Pcc1,Kae1,Bud32,Cgi121,and Gon7 in eukaryotes and is primari... Kinase,putative Endopeptidase,and Other Proteins of Small size(KEOPS)is a multisubunit protein complex conserved in eukaryotes and archaea.It is composed of Pcc1,Kae1,Bud32,Cgi121,and Gon7 in eukaryotes and is primarily involved in N^(6)-threonylcarbamoyl adenosine(t^(6)A)modification of transfer RNAs(tRNAs).Recently,it was reported that KEOPS participates in homologous recombination(HR)repair in yeast.To characterize the KEOPS in archaea(aKEOPS),we conducted genetic and biochemical analyses of its encoding genes in the hyperthermophilic archaeon Saccharolobus islandicus.We show that aKEOPS also possesses five subunits,Pcc1,Kae1,Bud32,Cgi121,and Pcc1-like(or Gon7-like),just like eukaryotic KEOPS.Pcc1-like has physical interactions with Kae1 and Pcc1 and can mediate the monomerization of the dimeric subcomplex(Kae1-Pcc1-Pcc1-Kae1),suggesting that Pcc1-like is a functional homolog of the eukaryotic Gon7 subunit.Strikingly,none of the genes encoding aKEOPS subunits,including Pcc1 and Pcc1-like,can be deleted in the wild type and in a t^(6)A modification complementary strain named TsaKI,implying that the aKEOPS complex is essential for an additional cellular process in this archaeon.Knock-down of the Cgi121 subunit leads to severe growth retardance in the wild type that is partially rescued in TsaKI.These results suggest that aKEOPS plays an essential role independent of the cellular t^(6)A modification level.In addition,archaeal Cgi121 possesses dsDNA-binding activity that relies on its tRNA 3ʹCCA tail binding module.Our study clarifies the subunit organization of archaeal KEOPS and suggests an origin of eukaryotic Gon7.The study also reveals a possible link between the function in t^(6)A modification and the additional function,presumably HR. 展开更多
关键词 ARCHAEA dna homologous recombination repair Gon7 KEOPS t^(6)A modification
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Regulatory issues for genetically modified animals 被引量:3
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作者 Perry Bradbury HACKETT 《Frontiers of Agricultural Science and Engineering》 2020年第2期188-203,共16页
Precision genetics and breeding have the potential to meet the agricultural needs and goals of the world in the 21 st century.These needs include increasing the efficiency of production of animals and improving their ... Precision genetics and breeding have the potential to meet the agricultural needs and goals of the world in the 21 st century.These needs include increasing the efficiency of production of animals and improving their products with minimal impact on the environment.The USA is the major innovator in genomic science and the acknowledged leader in formulating policies to regulate genetic applications in medicine and agriculture.However,governments worldwide have been exceedingly reluctant to support the introduction of genetically modified(GM)animals into agriculture.Regulatory policies have stagnated due to legal guidelines that could not anticipate the needs and solutions that are evident today.This must change if we are to maintain planetary integrity.I propose a new,market-based regulatory model for GM livestock that has both a strong scientific foundation and has worked for 10000 years.The model is similar to that for information technology in which specific algorithms drive computer and cell phone applications.Genome engineers write genetic algorithms that drive the traits in biological organisms.Accordingly,GM products should be viewed in terms of their use and public benefit rather than by limitations to the genetic programing coming from a few highly vocal groups.Genetic algorithms(Genapps)of the 21st century will include not only introduction of synthetic genes,but also complete natural and synthetic biochemical pathways to produce agricultural products that are maximally efficient,healthy to humans and animals,and sustainable in an era of changing climates while avoiding environmental degradation. 展开更多
关键词 algorithms EDITING FDA GMO recombinant dna USDA
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Expression of TIMP-3 Gene by Construction of a Eukaryotic Cell Expression Vector and Its Role in Reduction of Metastasis in a Human Breast Cancer Cell Line 被引量:11
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作者 XichunHan HongZhang +2 位作者 MingkuJia GangHan WeidongJiang 《Cellular & Molecular Immunology》 SCIE CAS CSCD 2004年第4期308-310,共3页
The present study is aimed at studying the gene for TIMP-3,a mammalian tissue inhibitor,by constructing a recombinant eukaryotic cell vector for gene therapy in human breast cancer.We obtained the TIMP-3 gene from the... The present study is aimed at studying the gene for TIMP-3,a mammalian tissue inhibitor,by constructing a recombinant eukaryotic cell vector for gene therapy in human breast cancer.We obtained the TIMP-3 gene from the human placent by RT-PCR.TIMP-3 gene was subcloned into pcDNA3.1 vetor from pMD18T vector by means of gene cloning to construct pcDNA3.1 recombinant vector.Human breast cancer cell line MDA-MB-453 was transfected with pcDNA3.1-TIMP3 recombinant vector using lipofectamine reagent.Then the expression of TIMP-3 and the effect on the metastasis of MDA-MB-453 were examined.The correct construction of pcDNA-TIMP3 was identified by means of restriction enzyme analysis,PCR amplication and nucleotide sequencing.Western blotting showed that the transfected cells were able to express TIMP-3, indicating that our construction of the pcDNA-TIMP3 eukaryotic expression vector was constructed successfully.Our experiments further indicated that the potential of metastasis was significantly reduced for the transfected cell line MDA-MB-453.Cellular & Molecular Immunology.2004;1(4):308-310. 展开更多
关键词 TIMP-3 gene eukaryotic expression dna recombinant technology TRANSFECTION
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重组变应原在特异性免疫治疗中的应用 被引量:1
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作者 王俊阁 王学艳 《国际耳鼻咽喉头颈外科杂志》 2014年第4期241-245,共5页
免疫治疗是治疗变应性疾病的根本措施,重组变应原就是利用重组DNA技术对已明确致敏蛋白组分的变应原构建变异体,其特性就是保持变应原的免疫特性,降低IgE结合活性.目前,已有几百种变应原有了重组变应原,重组变应原在临床诊断和评价患者... 免疫治疗是治疗变应性疾病的根本措施,重组变应原就是利用重组DNA技术对已明确致敏蛋白组分的变应原构建变异体,其特性就是保持变应原的免疫特性,降低IgE结合活性.目前,已有几百种变应原有了重组变应原,重组变应原在临床诊断和评价患者的致敏状况方面已成为一种很好的方法;对用于皮下和舌下免疫治疗的适宜性还有待于进行评估.本文就重组变应原的优点、基本特性、低变应原性、单一变应原制剂和复合变应原制剂的临床研究进展、个性化免疫治疗进行综述. 展开更多
关键词 变应原(Allergen) dna 重组(dna recombinant) 抗体(Antibodies) 免疫疗法(Immunotherapy)
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