白血病细胞株KG-1中Mxi1基因突变的检测和表达载体的构建

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山东大学学报(医学版) ›› 2011, Vol. 49 ›› Issue (10): 89-.

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白血病细胞株KG-1中Mxi1基因突变的检测和表达载体的构建

郭晓玲1,张改玲1,尹风雷1,牛志云1，张学军1,董作仁1，朱平2，潘崚1

1.河北医科大学第二医院血液内科，河北省血液病重点实验室, 石家庄 050000；
2.北京大学第一医院血液科，北京 100034

收稿日期:2011-04-08 出版日期:2011-10-10 发布日期:2011-10-10
通讯作者: 潘崚 (1962- )，主任医师,博导，主要从事恶性血液病基因诊断及治疗的研究。Email：13932113351@163.com
作者简介:郭晓玲(1972- )，副主任医师,副教授，博士，主要从事恶性血液病基因诊断及治疗的研究。
基金资助:
河北省自然科学基金资助项目(C2008001097)，国家高等学校博士学科点专项科研基金资助项目(200800890011)

Detection of the Mxi1 gene mutation and construction of the expression vector in the leukemia cell line KG-1

GUO Xiao-ling1， ZHANG Gai-ling1， YIN Feng-lei1， NIU Zhi-yun1，
ZHANG Xue-jun1， DONG Zuo-ren1， ZHU Ping2， PAN Ling1

1. Department of Hematology, The Second Hospital of Hebei Medical University, Hebei Province Key Laboratory of Hematopathy, Shijiazhuang 050000, China;
2. Department of Hematology, The First Hospital of Peking University， Beijing 100034, China

Received:2011-04-08 Online:2011-10-10 Published:2011-10-10

摘要/Abstract

摘要：

目的检测白血病细胞株KG-1中Mxil基因SID和bHLHzip区突变情况并构建Mxi1基因的野生型和突变型真核表达载体，观察其转染真核细胞后基因表达的情况。方法应用RT-PCR和SSCP分析KG-1细胞株Mxil基因的突变，将Mxi1野生型/突变型基因cDNA插入到pDs-red2-N1质粒中，构建pDs-red2-N1/Mxi1(野生型/突变型)真核表达载体，采用脂质体方法将质粒转染COS-7细胞，流式细胞仪检测红色荧光蛋白表达并计算转染效率。RT－PCR检测转染后Mxi1基因的表达。结果 Mxi1基因突变位于Helix II区第82编码子的CAT/TAT(His/Tyr)。成功构建pDs-red2-N1/Mxi1(野生型/突变型)真核表达载体，经酶切、电泳可以看到在4700、1845bp存在两条电泳条带， Mxi1基因在COS7细胞中得到表达，转染后COS-7细胞红色荧光蛋白表达的阳性细胞为18.07％，表达高峰出现在转染后第3天，并可持续表达6d左右。结论 Mxi1基因的高度保守区域bHLHzip存在基因突变，Mxi1突变基因的真核表达载体构建成功，并成功转染真核细胞COS-7

关键词: 基因，mxi1；基因，myc；载体构建；基因转染

Abstract:

Objective To detect mutation in Sin3-interacting domain(SID) and basic helix-loop-helix leucine zipper domain(bHLHzip) of the Mxi1 gene in the leukemia cell line KG-1, and construct a eukaryotic expression vector of Mxi1, and observe expression of the Mxi1 gene after being transfected into eukaryotic cells. Methods Expression and mutation of the Mxi1 gene in the leukemia cell line KG-1 were analyzed by reverse transcription-polymerase chain reaction(RT-PCR), single strand conformational po-lymorphism (SSCP) and DNA sequencing. The full length cDNA of the Mxi1 gene was inserted into the plasmid pDs-red2-N1 obtained from fetal lymphocytes and KG-1 cells，which was named pDs-red2-N1/Mxi1(wild /mutation type). Then the vector was transfected into COS-7 cells via liposomes. The Mxi1 mRNA expression was detected by RT-PCR and Mxi1 protein expression was detected by flow cytometry and a fluorescence microscope in COS-7 cells after transfection. Results DNA sequencing showed the 82th code CAT/TAT(His/Tyr) missense mutation in Helix II region in the KG-1 cell line. After the pDs-red2-N1/Mxi1 eukaryotic expressionvector was digested by endonuclease，two fragments of 4700bp and 1845bp in electrophoresis gel were detected. Expression of the Mxi1 gene could be found in COS-7 cells . The positive cell rate reached about 18.07% after transfection. Mxi1 expression lasted about 6 days in COS-7 cells and the peak occurred on the third day. Conclusion Mxi1 mutation occurs in the highly conserved domain bHLHzip in the KG-1 cell line. The Mxi1 gene eukaryotic expression vector was successfully constructed and transfected into COS-7 cells.

Key words: Genes, mxi1; Genes, myc； Vector construction; Gene transfectionMyc

中图分类号:

R556．9

郭晓玲1,张改玲1,尹风雷1,牛志云1，张学军1,董作仁1，朱平2，潘崚1. 白血病细胞株KG-1中Mxi1基因突变的检测和表达载体的构建[J]. 山东大学学报(医学版), 2011, 49(10): 89-.

GUO Xiao-ling1， ZHANG Gai-ling1， YIN Feng-lei1， NIU Zhi-yun1， ZHANG Xue-jun1， DONG Zuo-ren1， ZHU Ping2， PAN Ling1. Detection of the Mxi1 gene mutation and construction of the expression vector in the leukemia cell line KG-1[J]. JOURNAL OF SHANDONG UNIVERSITY (HEALTH SCIENCES), 2011, 49(10): 89-.

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