基因芯片表达谱筛选Kaposi肉瘤相关基因

Abstract

Abstract:

Objective To screen for Kaposi sarcoma （KS）-related genes. Methods Tissue samples were obtained from the lesion and normal skin of a patient with KS in Xinjiang Uygur Autonomous Region, and total RNA was extracted from these samples and reverse transcribed into cDNA. Real-time fluorescent quantitative reverse transcription PCR （RT-qPCR） was performed to determine the expression of K8.1, K2 and ORF50 in these samples. The cDNA was labeled with fluorescein and hybridized to a human 35K genome array containing 25 100 genes. Subsequently, the signal images were scanned by a laser scanner and acquired images were analyzed by software. Results RT-qPCR revealed the mRNA expression of K8.1, K2 and ORF50 in the KS tissues but not in the normal skin tissues, indicating that there was no crossed contamination in these specimens. Among the 25 100 genes, 1313 genes were identified to be differentially expressed between KS and normal skin tissues, including 756 up-regulated genes and 557 down-regulated genes. These differentially expressed genes, such as myeloid cell leukemia-1 gene （MCI-1）, annexins （ANX） and serine proteinase inhibitor Kazal type 5 （SPINK5）, were associated with apoptosis, angiogenesis, cell signaling, protein processing, cell cycle regulation, and so on. Conclusion The differentially expressed genes such as MCI-1 and SPINK5 may be associated with the development of KS.

Key words: Differential expression gene

References

[1] Antman K, ChangY. Kapod’s sarcoma[J]. The N Eng J Med, 2000, 342: 1027-1036. [2] Dilnur P, Katano H, Wang ZH, et al. Classic type of Kaposi's sarcoma and human herpesvirus 8 infection in Xinjiang, China. Pathol Int, 2001, 51: 845-52. [3] He F, Wang X, He B, et al. Human herpesvirus 8: serovprevalence and correlates in tumor patients from Xinjiang, China. J Med Virol, 2007, 79: 161-6. [4] 谭晓华，杨磊. 病毒感染在卡波氏肉瘤发病中的作用研究进展. 中国公共卫生，2004，20:1511-1513. [5] 李曼，赵作伟，辛彦. 应用基因表达谱芯片筛选胃腺癌相关基因. 世界华人消化杂志，2006，14: 666-670. [6] 徐益明，普雄明，李锋. 新疆 kaposi 肉瘤 43 例临床及病理学分析. 中国麻风皮肤病杂志，2005，21: 685-687. [7] 左学兰，周新，杨华强，等. B细胞非霍奇金淋巴瘤中MC1-1和p63表达的临床意义. 中华检验医学杂志，2006，29: 841-843. [8] 陈霞，李旭，陈葳. MCL-1基因研究新进展. 国外医学遗传学分册，2003，26: 148-151. [9] Gouill SI, Podar K, Amiot M, et al. VEGF induces MCI-l up regulation and protects multiple myeloma celIs against apoptosis. Blood, 2004, 104: 2886-2892. [10] 谢丽，陈晓燕，秦雪. Annexins 与肿瘤的相关研究. 医学综述，2007，13: 196-198. [11] TZIVION G, GUPTA V S. 14-3-3 proteins as potential oncogenes. Sem in Cancer Biol, 2006, 16: 203-213. [12] 曾妍，杨磊，仙玲玲. 实时荧光 PCR检测14-3-3β基因在新疆经典型 Kaposi肉瘤中的表达. 医学研究杂志，2007，36: 35-38. [13] Rodriguez JC, Diaz M, Gonzalez LO, et al. Apolipoprotein D expression in benign and malignant prostate tissues. Int J Surg Investig, 2000, 2: 319-326. [14] Sarjeant JM, Lawrie A, Kinnear C, et al. Apolipoprotein D inhibits platelet-derived growth factor-BB-induced vascular smooth muscle cell proliferated by preventing translocation of phosphorylated extracellular signal regulated kinase 1/2 to the nucleus. Arterioscler Thromb Vasc Biol, 2003, 23: 2172-2177. [15] Alvarez ML, Barbon JJ, Gonzalez LO, et al. Apolipoprotein D expression in retinoblastoma. Ophthalmic Res, 2003, 35: 111-116. [16] 徐敏，纪岩文. 特应性皮炎基因位点及基因治疗进展. 国际皮肤性病学杂志，2007，33: 98-100.

Screening for Kaposi sarcoma-associated genes by using Genechip technology

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