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Diversity of Microflora in Colonic Mucus from Severe Ulcerative Colitis Patients Analyzed by Terminal Restriction Fragment Length Polymorphism and Clone Libraries of Bacterial 16S rRNA Gene Sequences 被引量:1
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作者 I-Nung Huang Yuri Sato +8 位作者 Mitsuo Sakamoto Moriya Ohkuma Shinobu Ohnuma Takeshi Naitoh Chikashi Shibata Akira Horii Junko Nishimura Haruki Kitazawa Tadao Saito 《Advances in Microbiology》 2014年第13期857-870,共14页
Although the gut microflora is thought to be an essential factor in the development of ulcerative colitis (UC), the entire gut microflora occurring in UC remains unknown. Most studies use feces to represent the microf... Although the gut microflora is thought to be an essential factor in the development of ulcerative colitis (UC), the entire gut microflora occurring in UC remains unknown. Most studies use feces to represent the microflora distribution;however, here we analyzed the bacterial diversity in colonic mucus from UC patients receiving colectomy surgery and control patients. The diversity of microflora was investigated using a combination of terminal restriction fragment length polymorphism (T-RFLP) and clone library analyses of the 16S rRNA gene sequences. In the T-RFLP analysis, the number of terminal restriction fragments (T-RFs) decreased significantly in UC patients when compared to control samples. Also in the clone library analysis, the number of operational taxonomic units (OTU) and the Shannon diversity index were reduced significantly in UC patients. These molecular analyses reveal an overall dysbiosis in UC patients. No specific pathogen was found, and a strong negative correlation in relative abundance of bacterial populations was observed between the phyla Bacteroidetes and Firmicutes in the UC patients. This is the first report showing a significant correlation between these two phyla, which may be important characteristics in the pathogenesis of UC. 展开更多
关键词 ULCERATIVE Colitis MICROFLORA terminal restriction fragment length polymorphism 16S rRNA Gene CLONE Library
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Development of Fok-I based nested polymerase chain reaction-restriction fragment length polymorphism analysis for detection of hepatitis B virus X region V5M mutation 被引量:2
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作者 Hong Kim Seok-Hyun Hong +2 位作者 Seoung-Ae Lee Jeong-Ryeol Gong Bum-Joon Kim 《World Journal of Gastroenterology》 SCIE CAS 2015年第47期13360-13367,共8页
AIM: To develop a Fok-I nested polymerase chain reaction(PCR)-restriction fragment length polymorphism analysis(PRA) method for the detection of hepatitis B virus X region(HBx) V5 M mutation.METHODS: Nested PCR was ap... AIM: To develop a Fok-I nested polymerase chain reaction(PCR)-restriction fragment length polymorphism analysis(PRA) method for the detection of hepatitis B virus X region(HBx) V5 M mutation.METHODS: Nested PCR was applied into DNAs from 198 chronic patients at 2 different stages [121 patients with hepatocellular carcinoma(HCC) and 77 carrier patients]. To identify V5 M mutants, digestion of nested PCR amplicons by the restriction enzyme Fok-I(GGA TGN9↓) was done. For size comparison, the enzymetreated products were analyzed by electrophoresis on 2.5% agarose gels, stained with ethidium bromide, and visualized on a UV transilluminator.RESULTS: The assay enabled the identification of 69 patients(sensitivity of 34.8%; 46 HCC patients and 23 carrier patients). Our data also showed that V5 M prevalence in HCC patients was significantly higher than in carrier patients(47.8%, 22/46 patients vs 0%, 0/23 patients, P < 0.001), suggesting that HBx Ag V5 M mutation may play a pivotal role in HCC generation in chronic patients with genotype C infections.CONCLUSION: The Fok-I nested PRA developed in this study is a reliable and cost-effective method to detect HBx Ag V5 M mutation in chronic patients with genotype C2 infection. 展开更多
关键词 Hepatitis B virus X ANTIGEN Polymerasechain reaction-restriction fragment length polymorphismanalysis V5M MUTATION Hepatocellur carcinoma
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Antibiotic-Resistant Bacterial Group in Field Soil Evaluated by a Newly Developed Method Based on Restriction Fragment Length Polymorphism Analysis 被引量:1
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作者 Katsuji Watanabe Naoto Horinishi Kunimasa Matumoto 《Advances in Microbiology》 2015年第12期807-816,共10页
Spreading of antibiotic resistant bacteria into environment is becoming a major public health problem, implicating affair of the indirect transmission of antibiotic resistant bacteria to human through drinking water, ... Spreading of antibiotic resistant bacteria into environment is becoming a major public health problem, implicating affair of the indirect transmission of antibiotic resistant bacteria to human through drinking water, or vegetables, or daily products. Until now, the risk of nosocomial infection of antibiotic resistant bacteria has mainly been evaluated using clinical isolates by phenotypic method. To evaluate a risk of community-acquired infection of antibiotic resistant bacteria, a new method has been developed based on PCR-RFLP without isolation. By comparing restriction fragment lengths of the 16S rDNA gene from bacterial mixture grown under antibiotic treatment to those simulated from the DNA sequence, bacterial taxonomies were elucidated using the method of Okuda and Watanabe [1] [2]. In this study, taxonomies of polymyxin B resistant bacteria group in field soils, paddy field with organic manure and upland field without organic manure were estimated without isolation. In the both field soils, the major bacteria grown under the antibiotic were B. cereus group, which had natural resistance to this antibiotic. In field applied with organic manure, Prevotella spp., and the other Cytophagales, which were suggested to be of feces origin and to acquire resistance to the antibiotic, were detected. When numbers of each bacterial group were roughly estimated by the most probable number method, B. cereus group was enumerated to be 3.30 × 106 MPN/g dry soil in paddy field soil and 1.32 × 106 MPN/g dry soil in upland filed. Prevotella spp. and the other Cytophagales in paddy field were enumerated to be 1.31 × 106 MPN, and 1.07 × 106 MPN·g-1 dry soil. 展开更多
关键词 POLYMYXIN B Resistant Bacteria Field Soil Microchip ELECTROPHORESIS Multiple Enzyme restriction fragment length polymorphism Analysis the Most PROBABLE Number METHOD
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RESTRICTION FRAGMENT LENGTH POLYMORPHISMS ASSOCIATED WITH FACTOR Ⅷ CARRIER DETECTION USING DNA RFLPs IN CHINESE
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作者 汪运山 王德芬 曾畿生 《Medical Bulletin of Shanghai Jiaotong University》 CAS 1992年第2期28-34,共7页
RFLPs for XbaI, BelI and BglI sites of human FⅧwere informative for 48%, 41% and 15% of females studied, respectively. BglI RFLP is different from that reported by Chan et al, a fact suggests Yangtze River region pop... RFLPs for XbaI, BelI and BglI sites of human FⅧwere informative for 48%, 41% and 15% of females studied, respectively. BglI RFLP is different from that reported by Chan et al, a fact suggests Yangtze River region population of China would be at variance with the Southern Chinese population in certain RFLP distribution. TaqI allelic system Ⅰin the DXS52 region also shows the same variance among them, but heterozygous rate 0f 71% for system Ⅰ(alleles 1 to 8) and 49% for system Ⅱ(αand βalleles) were very similar. Using the Bell/XbaI RFLPs, accurate information could be obtained from this study for 56% of women who were at risk for hemophilia A (HA) carriership. The carrier of the remaining 44% could be determined by utilizing the TaqI RFLP. In addition, we report a new intergenie polymorphism (9%) at DXS115 as a marker for detection of heterozygotes in families at risk for HA. The advantage of using the XbaI/KpnI RFLP is that both the intragemie RFLP and the new intergenie RFLP can be evaluated on the same blot at the same time. 展开更多
关键词 restriction fragment length polymorphism HEMOPHILIA A CARRIER detection X CHROMOSOME allelic frequencies
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Comparing the frequencies of restriction fragment length polymorphisms for dystrophin gene in Chinese with those from Japanese and Caucasian populations^1
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作者 YULong MINQINWANG +4 位作者 QUNBINWANG WEIYIWANG YUMEIYANG JINGDEZHU SHOUYUANZHAO 《Cell Research》 SCIE CAS CSCD 1993年第1期38-38,40-47,共9页
The restriction fragment length polymorphisms distribution and frequency of dystrophin gene in Chinese were studied by using 14 subeiones of the entire 14kb eDNA for the dystrophin as hybridization probes. Allelie fra... The restriction fragment length polymorphisms distribution and frequency of dystrophin gene in Chinese were studied by using 14 subeiones of the entire 14kb eDNA for the dystrophin as hybridization probes. Allelie fragments were detected in hybridization patterns of PvuⅡ/la. TaqⅠ/2b-3, Taq Ⅰ/5b-7. and Xba Ⅰ/10. Among them. the allelic fragments (26kb and 3.8kb) in PvuⅡ/2b-3 pattern and the allelic fragments (10.0kb and 8.4kb) in Taq Ⅰ/5b-7 patterns had never been reported previously. Compared with the data from Caucasians and Japanese. it indicated that here was a significant difference (P <0.01) of the allelic fragment frequency in Taq Ⅰ/2b-3 and Xba Ⅰ/10 patterns between Chinese and Caucasians. The frequencies of allelic fragments A2 (5.6kb) in Taq Ⅰ/8 and A2 (10.7kb) in EcoR V/9 were high in Caucasians, yet had not been detected in Chinese, the differences were also highly significant. But in Chinese and Caucasians. the BIB2 allelic frequencies in Taq Ⅰ/5b-7 are the same. As to the frequency of the allelic fragments A1A2 and B1B2 in Pvu Ⅱ/1a. there was no significant difference between Chinese and Japenese. 展开更多
关键词 营养不良基因 基因频率 中国人 日本人 高加索人 RFLP 比较研究
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Bacterial Groups Concerned with Maturing Process in Manure Production Analyzed by a Method Based on Restriction Fragment Length Polymorphism Analysis
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作者 Katsuji Watanabe Naoto Horinishi +2 位作者 Kunimasa Matumoto Akihiro Tanaka Kenichi Yakushido 《Advances in Microbiology》 2015年第13期832-841,共10页
Composting is a biological aerobic decomposition process consisted from different phases. Although the Japanese Standards for manure recommended that it took at least 6 months to complete the maturing phase, there was... Composting is a biological aerobic decomposition process consisted from different phases. Although the Japanese Standards for manure recommended that it took at least 6 months to complete the maturing phase, there was no reliable ground. In order to find out shortening method of the maturing phase, the microorganisms concerned with a progress of the maturing was determined by using the most probable number method (MPN) and PCR-RFLP of the 16S rDNA, which was found effective to provide numbers and taxonomy of polymyxin B resistant bacterial groups in the former paper [1]. Compared to the numbers after thermophilic phase, those of Actinobacteria, δ-proteobacteria, and the other gram negative bacteria increased to 50 times, 20 times, and 105 times, respectively, after maturing phase, while those of Bacillus spp., and α and β-proteobacteria decreased to 1/10, and 1/105 after maturing phase. Numbers of the other Fumicutes, and γ-proteobacteria remained in the same revel. Actinobacteria, δ-proteobacteria, and the other gram negative bacteria might be concerned with a progress of the maturing phase, because these bacterial groups were detected and enumerated due to their proliferation ability. Although number of Acitinobacteria might be underestimated because of a PCR bias, the method was found effective for the purpose to monitor bacteria actively proliferated in culture medium. 展开更多
关键词 Maturing Phase MANURE PRODUCTION Microchip ELECTROPHORESIS Multiple Enzyme restriction fragment length polymorphism Analysis The Most PROBABLE Number METHOD
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Genotyping of human platelet antigen (HPA) system 5 of Chinese Han population in Shanghai by PCR restriction fragment length polymorphism(PCRRFLP)
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《中国输血杂志》 CAS CSCD 2001年第S1期376-,共1页
关键词 PCRRFLP length Genotyping of human platelet antigen system 5 of Chinese Han population in Shanghai by PCR restriction fragment length polymorphism HPA
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Evaluation of the Method Based on Restriction Fragment Length Polymorphism Analysis as Simple Analysis Method of Lactic Acid Bacteria in Foods
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作者 Kunimasa Matsumoto Kouya Shimada +1 位作者 Naoto Horinishi Katsuji Watanabe 《Food and Nutrition Sciences》 2016年第3期163-172,共10页
Lactic acid bacteria have not only been used to produce various kinds of fermented food, but also used as probiotic products. As lactic acid bacterial group was consisted from diverse genera, a simple inspection metho... Lactic acid bacteria have not only been used to produce various kinds of fermented food, but also used as probiotic products. As lactic acid bacterial group was consisted from diverse genera, a simple inspection method by which numbers and contained microorganisms could be automatically analyzed without any preliminary information was required to use them more effectively. In this manuscript, lactic acid bacterial groups in commercial products of kimuchi, komekouji-miso, and yoghurt were identified and enumerated by our newly developed method [1]-[3], to evaluate whether the method could be used as an inspection method of various food samples. In kimuchi, numerically dominant bacteria were Lactobacillus sakei, and L. casei (1.4 × 104 MPN g<sup>-1</sup>) and Leuconostoc spp. (l.4 × 104 MPN). In kouji-miso, numerically dominant bacteria was Bacillus spp. (3 × 103 MPN), which mainly included B. subtilis group and B. cereus group. Lactic acid bacteria such as Lactobacillus spp., or Lactococcus spp., included in the komekouji-miso, could be enumerated after 3 days incubation (1.24 × 104 MPN), but not detected after 7 days incubation. In yoghurt A and C, Lactococcus lactis was detected as numerically dominant lactic acid bacteria (3.0 × 105 MPN). In yoghurt B, Lactobacillus spp., or Lactococcus spp., was detected not only by a culturebased method but also by an unculture-based method, although there was a difference between the both estimated numbers. The present results suggested that the method might become useful as a simple inspection method of food microorganisms, because time and labor of the analysis could be reduced by using an unculture-based method and MCE-202 MultiNA. In this study, Bifidobacteriium spp. was not detected in B and C yoghurt, in spite of indicating their existence, and numbers of lactic acid bacteria were lower than the level of the daily product regulation, because 16S rDNA of Bifidobacteriium spp. might not be amplified by the used PCR condition. The PCR condition must be changed so as to amplify Bifidobacterium spp., before the method will be used as an inspection method for lactic acid bacteria. 展开更多
关键词 Multiple Enzyme restriction fragment length polymorphism Analysis Most Probable Number Method Lactic Acid Bacteria Komekouji-Miso Kimuchi YOGHURT
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RESTRICTION FRAGMENT LENGTH POLYMORPHISM(RFLP) ANALYSIS OF GENOMIC DNA OF 5 STRAINS OF TRICHINELLA SPIRALIS IN CHINA
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作者 王虹 张月清 +1 位作者 劳为德 吴赵永 《Chinese Medical Sciences Journal》 CAS CSCD 1995年第3期131-135,共5页
RESTRICTIONFRAGMENTLENGTHPOLYMORPHISM(RFLP)ANALYSISOFGENOMICDNAOF5STRAINSOFTRICHINELLASPIRALISINCHINAWangHon... RESTRICTIONFRAGMENTLENGTHPOLYMORPHISM(RFLP)ANALYSISOFGENOMICDNAOF5STRAINSOFTRICHINELLASPIRALISINCHINAWangHong(王虹)ZhangYueqing... 展开更多
关键词 RFLP 旋毛虫 DNA 寄生虫 基因组
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Differentiation of Helicobacter pylori isolates by polymerase chain reaction-restriction fragment length polymorphism
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作者 施理 孙勇 +2 位作者 张亚力 张振书 周殿元 《Journal of Medical Colleges of PLA(China)》 CAS 2002年第1期14-16,共3页
Objective: To investigate the association between the diversity of urease gene and urease activity of clinical isolates of Helicobacter pylori (H. pylori). Methods: Polymerase chain reaction-restriction fragment lengt... Objective: To investigate the association between the diversity of urease gene and urease activity of clinical isolates of Helicobacter pylori (H. pylori). Methods: Polymerase chain reaction-restriction fragment length polymorphism (PCR-RFLP) of urease gene and rapid urease activity test were used to study the urease activity of different clinical isolates of H. pylori. Results: H. pylori clinical isolates were divided into 4 types according to their PCR-RFLP results of urease gene and urease activity. Type Ⅰ , possessing strong urease activity (0. 11) and presented 1 fragment of 1. 7 kb by PCR-RFLP, had close relations with gastric ulcer; type Ⅱ , with the weakest urease activity (0. 07) and 2 fragments (1. 3 and 0. 4 kb respectively) , was associated with duodenal bulb ulcer; type Ⅲ , with the strongest urease activity (0. 12) and 2 fragments (0. 4 and 0. 17 kb) with or without 1 fragment (0. 23 or 0. 37 kb) , was responsible for gastritis; type Ⅳ , with weak urease activity (0. 09) and 2 展开更多
关键词 幽门螺旋杆菌 PCR 限制片段长度多态性 株系多样化
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The Use of Restriction Fragment Length Polymorphism and Fluorescence in Situ Hybridization to Investigate Microbiota of Piglets after Feeding Oregano
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作者 Katrin Stelter Andreas Berk +4 位作者 Lutz Geue Stefanie Barth Petra Schlien Alexander Swidsinski Sven Danicke 《Food and Nutrition Sciences》 2014年第17期1628-1636,共9页
A total of 80 piglets (7.9 ± 1.0 kg) were used in a feeding experiment with dried oregano. The diets differed in their oregano content: 0 g, 2 g, 4 g and 8 g oregano/kg feed, corresponding to 0, 23.5, 46.9 and 93... A total of 80 piglets (7.9 ± 1.0 kg) were used in a feeding experiment with dried oregano. The diets differed in their oregano content: 0 g, 2 g, 4 g and 8 g oregano/kg feed, corresponding to 0, 23.5, 46.9 and 93.9 mg carvacrol/kg DM. After the experimental period of 5 weeks, 20 piglets of both extreme feeding groups were slaughtered: 10 animals of the control group and 10 animals of the group that received 8 g oregano/kg. Ingesta samples of jejunum, caecum and colon were collected and analyzed by FISH and PCR RFLP to compare the diversity of microbiota. The results showed no significant changes in microbiota in response to oregano. The patterns of the PCR-RFLP showed a similarity of 61.8% - 91.8% in both feeding groups. In conclusion, an effect of oregano on the in- testinal microbiota could not be shown under the methods used. 展开更多
关键词 PIGLETS Origanum vulgare L. Fluorescence in Situ Hybridization restriction fragment length polymorphism Intestinal Microorganisms
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ACE2 rs2074192位点多态性与非乙醇性脂肪性肝病易感性的相关性
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作者 赵守林 张梅 +2 位作者 赵真真 陈立震 宣世英 《青岛大学学报(医学版)》 CAS 2024年第1期39-42,共4页
目的探讨青岛地区人群血管紧张素转化酶2(ACE2)rs2074192位点多态性与非乙醇性脂肪性肝病(NAFLD)易感性的相关性。方法研究纳入NAFLD病人208例,健康查体者105例。收集受试者的血液标本,提取DNA,应用多聚酶链反应(PCR)检测ACE2基因rs2074... 目的探讨青岛地区人群血管紧张素转化酶2(ACE2)rs2074192位点多态性与非乙醇性脂肪性肝病(NAFLD)易感性的相关性。方法研究纳入NAFLD病人208例,健康查体者105例。收集受试者的血液标本,提取DNA,应用多聚酶链反应(PCR)检测ACE2基因rs2074192位点的基因型,比较ACE2 rs2074192位点基因型及等位基因频率在NAFLD组及对照组的分布差异。同时收集受试者的临床资料及实验室生化检查结果,比较不同基因型病人临床资料及实验室生化结果的差异。结果NAFLD组和对照组ACE2 rs2074192位点的基因型与等位基因分布差异均无统计学意义(P>0.05)。ACE2 rs2074192位点T等位基因女性携带者体质量指数高于未携带者,T等位基因男性携带者血清葡萄糖水平低于未携带者(t=-2.613、-3.195,P<0.05)。结论青岛地区人群ACE2 rs2074192位点多态性与NAFLD易感性无明显相关性。 展开更多
关键词 非酒精性脂肪性肝病 多态性 限制性片段长度 血管紧张素转换酶2 疾病遗传易感性
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PEAR1基因多态性与缺血性脑卒中复发易感性的关系研究
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作者 张云芳 聂晓改 +2 位作者 吉永 王祝君 彭传梅 《国际检验医学杂志》 CAS 2024年第7期776-779,784,共5页
目的分析血小板内皮聚集受体1(PEAR1)基因多态性与缺血性脑卒中复发的相关性,为防治缺血性脑卒中复发提供依据。方法选取该院神经内科门急诊和住院确诊为急性缺血性脑卒中的150例患者作为研究对象,根据是否为脑卒中复发分为初发脑卒中组... 目的分析血小板内皮聚集受体1(PEAR1)基因多态性与缺血性脑卒中复发的相关性,为防治缺血性脑卒中复发提供依据。方法选取该院神经内科门急诊和住院确诊为急性缺血性脑卒中的150例患者作为研究对象,根据是否为脑卒中复发分为初发脑卒中组(127例)和复发脑卒中组(23例)。应用聚合酶链反应-限制性片断长度多态性(PCR-RFLP)方法分析PEAR1基因rs12041331位点单核苷酸多态性,并测序验证基因型。结果初发脑卒中组和复发脑卒中组PEAR1基因rs12041331G>A位点GG、GA、AA基因型和G、A等位基因频率比较,差异有统计学意义(P<0.05);复发脑卒中组的年龄较初发脑卒中组高,差异有统计学意义(P<0.05)。Logistic回归分析显示,年龄、PEAR1基因rs12041331位点AA基因型与缺血性脑卒中复发有关,是缺血性脑卒中复发的危险因素(P<0.05)。结论PEAR1基因rs12041331G>A位点多态性与缺血性脑卒中复发相关。PEAR1基因纯合突变可能是缺血性脑卒中复发的危险因素,PEAR1基因可能是缺血性脑卒中复发风险预测的候选基因。 展开更多
关键词 缺血性脑卒中 单核苷酸多态性 聚合酶链反应-限制性片断长度多态性 等位基因
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POLYMORPHISMS OF THE HUMAN LIPOPROTEIN LIPASE GENE:POSSIBLE ASSOCIATION WITH LIPID LEVELS IN PATIENTS WITH CORONARY HEART DIS 被引量:7
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作者 叶平 裴兰 王士雯 《Chinese Medical Sciences Journal》 CAS CSCD 1996年第3期157-161,共5页
POLYMORPHISMSOFTHEHUMANLIPOPROTEINLIPASEGENE:POSSIBLEASSOCIATIONWITHLIPIDLEVELSINPATIENTSWITHCORONARYHEARTDI... POLYMORPHISMSOFTHEHUMANLIPOPROTEINLIPASEGENE:POSSIBLEASSOCIATIONWITHLIPIDLEVELSINPATIENTSWITHCORONARYHEARTDISEASEINBEIJINGARE... 展开更多
关键词 脂蛋白酶 冠心病 基因多态性 心肌梗死 RFLPS
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Clinical significance of telomerase and its associate genes expression in the maintenance of telomere length in squamous cell carcinoma of the esophagus 被引量:6
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作者 Chung-Ping Hsu Li-Wen Lee +1 位作者 Sen-Ei Shai Chih-Yi Chen 《World Journal of Gastroenterology》 SCIE CAS CSCD 2005年第44期6941-6947,共7页
AIM: To observe the interaction between the expression of telomerase activity (TA) and its associate genes in regulation of the terminal restriction fragment length(TRFL) in esophageal squamous cell carcinoma (SCC).ME... AIM: To observe the interaction between the expression of telomerase activity (TA) and its associate genes in regulation of the terminal restriction fragment length(TRFL) in esophageal squamous cell carcinoma (SCC).METHODS: Seventy-four specimens of esophageal SCC were examined. The TA was measured by telomeric repeat amplification protocol (TRAP) assay, and the associated genes [human telomerase-specific reverse transcriptase (hTERT), hTERC, TP1, c-Myc, TRF1,and TRF2] were detected using RT-PCR method. The TRFL was measured by Telomere Length Assay Kit and Southern blotting. The correlations between the expression of telomerase and its associated genes with the TRFL and survivals were examined.RESULTS: Expressions of the TA, hTERT, hTERC, TP1,c-Myc, TRF1, and TRF2 genes were observed in 85.1%,64.9%, 79.7%, 100.0%, 94.6%, 82.4%, and 91.9% of the tumor tissues, respectively. The TRFL of the tumor and normal esophageal tissues were 2.70±1.42 and 4.93±1.74 kb, respectively (P<0.0001). The TRFL of the telomerase positive and telomerase negative tumor tissues were 2.72±1.44 and 2.58±1.32 kb, respectively (P = 0.767).The TRFL ratios (TRFLR) of the telomerase positive and telomerase negative tumor tissues were 0.55±0.22 and 0.59±0.41, respectively (P = 0.742). The expression rates of h-TERT (P = 0.0002), hTERC (P<0.0001), and TRF1(P = 0.002) in the tumor tissues are higher than those of the normal paired tissues. Though TA is markedly activated in tumor tissues (P<0.0001), its expression is not related to clinicopathological parameters including gender, tumor differentiation, and TNM stages. The cumulative 4-year survival rates of telomerase positive and telomerase negative cases were 35.86% and 31.2%,respectively (P = 0.8442). The cumulative 4-year survival rates of patients with their TRFLR ≤85% and >85%were 38.7% and 15.7%, respectively (P = 0.1307).CONCLUSION: Though telomerase expression is not related to tumor stages and prognosis, our data support that the TA increased as the TRFL decreased,probably under the control of hTERT, hTERC, and TRF1.When telomerase expression was activated, only TRF2overexpression persisted to stabilize T-loop formation.Furthermore, as the TRFLR decreased to 85%, a trend of better prognosis was observed. Cox model analysis indicates a higher t/n TRFLR and distant metastasis are independent poorer prognostic factors (P = 0.035 and P = 0.042, respectively). 展开更多
关键词 端粒 基因表达 鳞状细胞癌 食管癌
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Association of TNF-α-238G/A and 308 G/A Gene Polymorphisms with Pulmonary Tuberculosis among Patients with Coal Worker’s Pneumoconiosis 被引量:12
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作者 HONG-MIN FAN ZHUO WANG +7 位作者 FU-MIN FENG KONG-LAI ZHANG JU-XIANG YUAN HONG SUI HONG-YAN QIU LI-HUA LIU XIAO-JUAN DENG JING-XUE REN 《Biomedical and Environmental Sciences》 SCIE CAS CSCD 2010年第2期137-145,共9页
Objectives Tumor necrosis factor-α (TNF-α) may play an important role in host’s immune response to mycobacterium tuberculosis (M. tuberculosis) infection. This study was to investigate the association of TNF-α gen... Objectives Tumor necrosis factor-α (TNF-α) may play an important role in host’s immune response to mycobacterium tuberculosis (M. tuberculosis) infection. This study was to investigate the association of TNF-α gene polymorphism with pulmonary tuberculosis (TB) among patients with coal worker’s pneumoconiosis (CWP). Methods A case-control study was conducted in 113 patients with confirmed CWP complicated with pulmonary TB and 113 non-TB controls with CWP. They were matched in gender, age, job, and stage of pneumoconiosis. All participants were interviewed with questionnaires and their blood specimens were collected for genetic determination with informed consent. The TNF-α gene polymorphism was determined with polymerase chain reaction of restriction fragment length polymorphism (PCR-RFLP). Frequency of genotypes was assessed for Hardy-Weinberg equilibrium by chi-square test or Fisher’s exact probability. Factors influencing the association of individual susceptibility with pulmonary TB were evaluated with logistic regression analysis. Gene-environment interaction was evaluated by a multiplicative model with combined OR. All data were analyzed using SAS version 8.2 software. Results No significant difference in frequency of the TNF-α-308 genotype was found between CWP complicated with pulmonary TB and non-TB controls (χ2=5.44, P=0.07). But difference in frequency of the TNF-α-308 A allele was identified between them (χ2=5.14, P=0.02). No significant difference in frequencies of the TNF-α-238 genotype and allele (P=0.23 and P=0.09, respectively) was found between cases and controls either, with combined (GG and AA) OR of 3.96 (95% confidence interval of 1.30~12.09) at the-308 locus of the TNF-α gene, as compared to combination of the TNF-α-238 GG and TNF-α-308 GG genotypes. Multivariate-adjusted odds ratio of the TNF-α-238 GG and TNF-α-308 GA genotypes was 1.98 (95% CI of 1.06~3.71) for risk for pulmonary TB in patients with CWP. There was a synergic interaction between the TNF-α-308 GG genotype and body mass index (OR=4.92), as well as an interaction between the TNF-α-308 GG genotype and history of BCG immunization or history of TB exposure. And, the interaction of the TNF-α-238 GG genotype and history of BCG immunization or TB exposure with risk for pulmonary TB in them was also indicated. Conclusions TNF-α-308 A allele is associated with an elevated risk for pulmonary TB, whereas TNF-α-238 A allele was otherwise. 展开更多
关键词 基因多态性 肺结核 TNF 肿瘤坏死因子-α 尘肺 煤工 患者 LOGISTIC回归分析
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Association between estrogen receptor β gene Rsa1 polymorphism and depressive disorder in peri-menopausal and menopausal women 被引量:3
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作者 于学文 任永惠 +4 位作者 李学成 高成阁 李芬 韩蓁 李旭 《Journal of Medical Colleges of PLA(China)》 CAS 2005年第2期102-105,共4页
Objective: To investigate estrogen receptor β (ERβ) gene Rsa1 polymorphism and concentration of estrogen, FSH and LH in serum in peri-menopausal and menopausal women with depressive disorder. Methods: Seventy-four p... Objective: To investigate estrogen receptor β (ERβ) gene Rsa1 polymorphism and concentration of estrogen, FSH and LH in serum in peri-menopausal and menopausal women with depressive disorder. Methods: Seventy-four peri-menopausal and menopausal women with depressive disorder met ICD-10 and CCMD-3 assessment criteria for depressive disorder were recruited. ERβ gene Rsa1 polymorphism was analyzed with PCR-RFLP. Serum levels of estrogen, FSH and LH were measured by magnetism-ELISA. Results: The respective frequency of ERβ gene Rsa1 polymorphism was no significant difference between women with depressive disorder and the healthy women (χ 2=1.106,P>0.05). The serum level of estrogen was lower in women with depressive disorder than in the healthy women (P<0.05). No difference was found for FSH and LH between two groups. Conclusion: ERβ gene Rsa1 polymorphism may be not associated with depressive disorder in the peri-menopausal and menopausal women. The serum level of estrogen is associated with depressive disorder in the peri-menopausal and menopausal women. 展开更多
关键词 雌激素受体Β 基因多态性 更年期综合症 抑郁症状 女性
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Analysis of polymorphisms in the promoter region of interleukin-1 β by restriction fragment length polymorphism-PCR 被引量:1
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作者 文爱清 王军 +2 位作者 冯凯 朱佩芳 蒋建新 《Chinese Journal of Traumatology》 CAS 2004年第5期271-274,共4页
Objective: To investigate the frequencies of -1470, (-511) and -31 single nucleotide polymorphisms (SNPs) in the promoter of IL-1β and its haplotype constitution in Chongqing population. Methods: One hundred and twel... Objective: To investigate the frequencies of -1470, (-511) and -31 single nucleotide polymorphisms (SNPs) in the promoter of IL-1β and its haplotype constitution in Chongqing population. Methods: One hundred and twelve healthy Chongqing people were enrolled in this study. Polymorphisms at -1470 (G to C), (-511) (T to C) and -31 (C to T) of IL-1β were genotyped with the method of restriction fragment length polymorphism (RFLP). Haplotype frequencies were analyzed by Arlequine software.Results: Frequencies of IL-1β -1470, -511 and -31 SNPs were (41.67)%, 50% and (45.33)%, respectively. Genotype frequencies of -1470 locus were (39.81)%, (37.04)% and (23.15)% for G/G, G/C and C/C respectively. As for T-511C SNP, genotype frequencies of (T/T), T/C and C/C were (29.91)%, (40.18)% and (29.91)%, respectively. Genotyping results of C/C, C/T, and T/T of -31 locus were (35.51)%, (38.32)% and (26.71)% respectively. Haplotype analysis found that there were mainly three haplotypes constituted by three SNPs, ie., G-T-C, C-T-C and G-C-T. Conclusions: Polymorphisms exist in the promoter of IL-1β in Chongqing population. Three SNPs locate in the same haplotype block. 展开更多
关键词 多态现象 白细胞间介素-1β 抑制作用 PCR 单核苷 基因
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Association of G+1688A Polymorphism of Platelet Endothelial Cell Adhesion Molecule-1 Gene with Myocardial Infarction in the Chinese Han Population 被引量:1
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作者 杨颖 程龙献 +3 位作者 Ripen Nsenga 何美安 常智堂 邬堂春 《Journal of Huazhong University of Science and Technology(Medical Sciences)》 SCIE CAS 2007年第5期520-523,共4页
In order to investigate the association of G+1688A(Ser563Asn) polymorphism of platelet endothelial cell adhesion molecule-1(PECAM-1) gene with myocardial infarction(MI) in the Chinese Han population,the G+1688A polymo... In order to investigate the association of G+1688A(Ser563Asn) polymorphism of platelet endothelial cell adhesion molecule-1(PECAM-1) gene with myocardial infarction(MI) in the Chinese Han population,the G+1688A polymorphism in PECAM-1 gene was detected by polymerase chain reaction-restriction fragment-length polymorphism(PCR-RFLP) method among 502 subjects,including 218 patients with MI and 284 controls.The results showed that there was significant difference in AA frequencies of genotype G+1688A polymorphism between case and control groups(39% vs 24%,P<0.001).A similar trend was observed on the allele frequencies(A/G:62% vs 49%,P<0.001).Among the subjects with high serum total cholesterol level or high systolic blood pressure level,the variant AA genotype was associated with high risk of MI(adjusted OR,2.13;95% CI,1.08-4.41 and adjusted OR,2.53;95%CI,1.63-3.63).The single nucleotide polymorphism(SNP) at position +1688 in the exon 8 of PECAM-1 gene was associated with MI and the allele A might be a risk factor for MI in the Chinese Han population. 展开更多
关键词 心肌梗塞 聚合酶链反应 血小板内皮细胞粘附分子 基因多态性
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RESTRICTION ENDONUCLEASE ANALYSIS OF MITOCHONDRIALDNA FROM HUMAN LUNG ADENOCARCINOMA CELLLINE SPC-A-1
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作者 胡义德 钱桂生 +3 位作者 陈维中 李淑平 王关嵩 毛宝龄 《Chinese Journal of Cancer Research》 SCIE CAS CSCD 1999年第4期253-256,共4页
Objective: TO understand the role of mitochondrialDNA (mtDNA) in carcinogenesis. Methods: single-stepmethod was used to isolate the mtDNA from humanlung adenocarcinoma cell line SPC-A-1. The mtDNAwas analyzed by restr... Objective: TO understand the role of mitochondrialDNA (mtDNA) in carcinogenesis. Methods: single-stepmethod was used to isolate the mtDNA from humanlung adenocarcinoma cell line SPC-A-1. The mtDNAwas analyzed by restriction fragment lengthpolymorphism (RFLP) with 11 kinds of restrictionendonuclease, which were Pvu II, Xho I, Pst I, EcoR I,BstE II, Hind III, Hpa i, Bcl i, EcoR V, Sea I and Xba I.Restriction map of mtDNA from SPC-A-1 cell wasobtained by the single and double-digestion method.Results: It was found that no variation at 32 restrictionsites could be detected in the coding region of mtDNAfrom SPC-A-1 cell line. But a new site was found atnucleotide 16276 (EcoR V) within the noncoding region.Conclusion: These results indicate that the primarystructure of gene coding region of mtDNA isolated fromSPC-A-1 cell is highly stable. While the major variationof nucleotide is probably located in the noncodingregion. 展开更多
关键词 Lung carcinoma MITOCHONDRIAL DNA restriction fragment length polymorphism MUTATION
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