首页> 美国卫生研究院文献>Journal of the Boston Society of Medical Sciences >Identification of monoclonal B-cell populations by rapid cycle polymerase chain reaction. A practical screening method for the detection of immunoglobulin gene rearrangements.

【2h】

Identification of monoclonal B-cell populations by rapid cycle polymerase chain reaction. A practical screening method for the detection of immunoglobulin gene rearrangements.

机译：通过快速循环聚合酶链反应鉴定单克隆B细胞群体。一种检测免疫球蛋白基因重排的实用筛选方法。

代理获取

本网站仅为用户提供外文OA文献查询和代理获取服务，本网站没有原文。下单后我们将采用程序或人工为您竭诚获取高质量的原文，但由于OA文献来源多样且变更频繁，仍可能出现获取不到、文献不完整或与标题不符等情况，如果获取不到我们将提供退款服务。请知悉。

页面导航

摘要
著录项
相似文献
相关主题

摘要

Alternatives to Southern blot hybridization for gene rearrangement analysis are being studied because of the time, labor, cost, and radioisotopes required for this technique. We have utilized a rapid, hot air, thermocycling polymerase chain reaction (PCR) system to examine various lymphoproliferative disorders for immunoglobulin heavy chain (IgH) gene rearrangements. This unique system amplifies DNA from 10 microliters samples placed in glass capillary tubes, over a total cycle time of about 30 minutes. Amplified bands are easily visualized on ethidium bromide-stained agarose gels. Forty-one monoclonal B-cell proliferations, 27 reactive lymphoid hyperplasias, 17 T-cell lymphomas and 3 cases of Hodgkin's disease were studied. All 88 cases were fully characterized by morphologic, immunophenotypic, and genotypic (Southern blot) analyses. Each case was separately evaluated by PCR with two primer pairs: 1) IgH variable region (VH) and IgH joining region (JH) and 2) bcl-2 and JH. Thirty-four of 41 monoclonal B-cell proliferations revealed a distinct band (within an expected base pair range) with 1 or both primer combinations supporting B-cell monoclonality; the other 7 cases were considered false negatives. The 47 entities without IgH gene rearrangements detectable by Southern analysis demonstrated no amplified product or a smear of amplified DNA with no distinct band. The overall specificity of PCR was 100%, and the sensitivity was 83% when directly compared with Southern blot analysis. Although its sensitivity is currently less than optimal, PCR is a rapid and practical screening method for the detection of IgH gene rearrangements. If a positive result is obtained no further analysis is required; however, if there is a negative result, standard Southern blot analysis should be performed to definitively exclude the presence of a monoclonal B-cell population in the sample.

机译：由于该技术需要时间，劳力，成本和放射性同位素，因此正在研究用于基因重排分析的Southern blot杂交的替代方法。我们已经使用了快速，热空气，热循环聚合酶链反应（PCR）系统来检查免疫球蛋白重链（IgH）基因重排的各种淋巴增生性疾病。这种独特的系统可在大约30分钟的总循环时间内扩增来自置于玻璃毛细管中的10微升样品的DNA。在溴化乙锭染色的琼脂糖凝胶上可以轻松看到扩增的条带。研究了41个单克隆B细胞增殖，27个反应性淋巴样增生，17个T细胞淋巴瘤和3例霍奇金病。通过形态学，免疫表型和基因型（Southern blot）分析对所有88例病例进行了充分表征。通过PCR用两个引物对分别评估每种情况：1）IgH可变区（VH）和IgH连接区（JH）和2）bcl-2和JH。 41个单克隆B细胞增殖中的34个显示出明显的条带（在预期的碱基对范围内），其中一种或两种引物组合支持B细胞单克隆性；其他7例被认为是假阴性。通过Southern分析可检测到的没有IgH基因重排的47个实体显示没有扩增产物或没有明显条带的扩增DNA涂片。直接与Southern blot分析相比，PCR的总体特异性为100％，灵敏度为83％。尽管目前它的灵敏度还不够理想，但是PCR是检测IgH基因重排的一种快速而实用的筛选方法。如果获得阳性结果，则无需进一步分析；但是，如果结果为阴性，则应进行标准Southern印迹分析以明确排除样品中存在单克隆B细胞群。

著录项

期刊名称 Journal of the Boston Society of Medical Sciences
作者
G. H. Segal; C. T. Wittwer; A. J. Fishleder; M. H. Stoler; R. R. Tubbs; C. R. Kjeldsberg;
展开▼
作者单位

展开▼
年(卷),期 1992(141),6
年度 1992
页码 1291–1297
总页数 7
原文格式 PDF
正文语种
中图分类
关键词

相似文献

外文文献
中文文献
专利

1. Evaluation of B-cell clonality in archival skin biopsy samples of cutaneous B-cell lymphoma by immunoglobulin heavy chain gene polymerase chain reaction. [J] . Lukowsky A, Marchwat M, Sterry W, Leukemia and lymphoma . 2006,第3期

机译：通过免疫球蛋白重链基因聚合酶链反应评估皮肤B细胞淋巴瘤档案皮肤活检样品中B细胞克隆性。
2. MYD88 L265P in Waldenstrom macroglobulinemia, immunoglobulin M monoclonal gammopathy, and other B-cell lymphoproliferative disorders using conventional and quantitative allele-specific polymerase chain reaction. [J] . Lian Xu, Zachary R Hunter, Guang Yang, Blood: The Journal of the American Society of Hematology . 2013,第11期

机译：MYD88 L265P在Waldenstrom巨球蛋白血症，免疫球蛋白M单克隆丙种球蛋白病和其他B细胞淋巴增生性疾病中，使用常规和定量等位基因特异性聚合酶链反应。
3. MYD88 L265P in Waldenstrom macroglobulinemia, immunoglobulin M monoclonal gammopathy, and other B-cell lymphoproliferative disorders using conventional and quantitative allele-specific polymerase chain reaction. [J] . Lian Xu, Zachary R Hunter, Guang Yang, Blood: The Journal of the American Society of Hematology . 2013,第11期

机译：MyD88 L265P在瓦尔德斯特罗姆大葡萄球菌血症，免疫球蛋白M单克隆术术，以及使用常规和定量等位基因特异性聚合酶链反应的其他B细胞淋巴抑制性疾病。
4. PCR-DHPLC (Polymerase Chain Reaction - Denaturing High Performance Liquid Chromatography): a potential novel method for rapid screening of mixed yeast populations [C] . Mathias Hutzler, Oliver Goldenberg European Brewery Convention Congress . 2007

机译：PCR-DHPLC（聚合酶链反应-变性高效液相色谱法）：一种快速筛选混合酵母种群的潜在新方法
5. Development of a rapid detection method of Salmonella spp. on chicken skin by real-time polymerase chain reaction. [D] . Carter, Melvin. 2008

机译：沙门氏菌快速检测方法的开发。通过实时聚合酶链反应在鸡皮上
6. A Rapid Polymerase Chain Reaction-Based Screening Method for Identification of All Expanded Alleles of the Fragile X (FMR1) Gene in Newborn and High-Risk Populations [O] . Flora Tassone, Ruiqin Pan, Khaled Amiri, 2008

机译：基于快速聚合酶链反应的筛选方法用于鉴定新生儿和高危人群中的脆弱X（FMR1）基因的所有扩展等位基因
7. A Rapid Polymerase Chain Reaction-Based Screening Method for Identification of All Expanded Alleles of the Fragile X (FMR1) Gene in Newborn and High-Risk Populations [O] . Tassone, Flora, Pan, Ruiqin, Amiri, Khaled, 2008

机译：基于快速聚合酶链反应的筛选方法，用于鉴定新生儿和高危人群中的脆弱X（FMR1）基因的所有扩展等位基因
8. Rapid Method for Detection and Identification of Flaviviruses by Polymerase ChainReaction and Nucleic Acid Hybridization. (Reannouncement with New Availability Information) [R] . Watts, D. M., Puri, B., Henchal, E. A., 1994

机译：聚合酶链反应和核酸杂交检测和鉴定黄病毒的快速方法。（重新公布新的可用性信息）

Identification of monoclonal B-cell populations by rapid cycle polymerase chain reaction. A practical screening method for the detection of immunoglobulin gene rearrangements.

摘要

著录项

相似文献

相关主题

期刊订阅