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Description and Characterization of a Novel Human Mast Cell Line for Scientific Study

机译:新型人类肥大细胞系用于科学研究的描述和表征

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摘要

Background: Laboratory of allergic diseases 2 (LAD2) human mast cells were developed over 15 years ago and have been distributed worldwide for studying mast cell proliferation, receptor expression, mediator release/inhibition, and signaling. LAD2 cells were derived from CD34+ cells following marrow aspiration of a patient with aggressive mastocytosis with no identified mutations in . Another aspiration gave rise to a second cell line which has recently been re-established (LADR). We queried whether LADR had unique properties for the preclinical study of human mast cell biology. Methods: LADR and LAD2 cells were cultured under identical conditions. Experiments examined proliferation, beta-hexosaminidase (β-hex) release, surface receptor and granular protease expression, infectivity with HIV, and gene expression. Results: LADR cells were larger and more granulated as seen with Wright–Giemsa staining and flow cytometry, with cell numbers doubling in 4 weeks, in contrast to LAD2 cells, which doubled every 2 weeks. Both LADR and LAD2 cells released granular contents following aggregation of FcεRI. LADR cells showed log-fold increases in FcεRI/CD117 and expressed CD13, CD33, CD34, CD63, CD117, CD123, CD133, CD184, CD193, and CD195, while LAD2 cells expressed CD33, CD34, CD63, CD117, CD133, CD193 but not CD13, CD123, CD184, or CD195. LADR tryptase expression was one-log-fold increased. LADR cell and LAD2 cell chymase expression were similar. Both cell lines could be infected with T-tropic, M-tropic, and dual tropic HIV. Following monomeric human IgE stimulation, LADR cells showed greater surface receptor and mRNA expression for CD184 and CD195. Expression arrays revealed differences in gene upregulation, especially for the suppressor of cytokine signaling (SOCS) family of genes with their role in JAK2/STAT3 signaling and cellular myelo ytomatosis oncogene (c-MYC) in cell growth and regulation. Conclusions: LADR cells are thus unique in that they exhibit a slower proliferation rate, are more advanced in development, have increased FcεRI/CD117 and tryptase expression, have a different profile of gene expression, and show earlier infectivity with HIV-BAL, LAV, and TYBE when compared to LAD2 cells. This new cell line is thus a valuable addition to the few FcεRI+ human mast cell lines previously described and available for scientific inquiry.
机译:背景:过敏性疾病2(LAD2)实验室人类肥大细胞建立于15年前,已分布于全世界,用于研究肥大细胞增殖,受体表达,介质释放/抑制和信号传导。 LAD2细胞来源于患有侵袭性肥大细胞增多症且未鉴定到突变的患者的骨髓抽吸后的CD34 +细胞。另一个愿望产生了第二个细胞系,该细胞系最近已重建(LADR)。我们询问LADR是否对人类肥大细胞生物学的临床前研究具有独特的特性。方法:在相同条件下培养LADR和LAD2细胞。实验检查了增殖,β-己糖胺酶(β-hex)释放,表面受体和颗粒蛋白酶表达,HIV感染性以及基因表达。结果:通过Wright–Giemsa染色和流式细胞仪观察,LADR细胞更大且颗粒更多,在4周内细胞数量翻了一番,而LAD2细胞每2周增加一倍。 FcεRI聚集后,LADR和LAD2细胞均释放出颗粒状内容物。 LADR2细胞显示FcεRI/ CD117的对数倍增加,并表达CD13,CD33,CD34,CD63,CD117,CD123,CD133,CD184,CD193和CD195,而LAD2细胞表达CD33,CD34,CD63,CD117,CD133,CD193,但不是CD13,CD123,CD184或CD195。 LADR类胰蛋白酶表达增加了1个对数。 LADR细胞和LAD2细胞的糜酶表达相似。两种细胞系都可以感染T-向性,M-向性和双重向性HIV。在单体人IgE刺激后,LADR细胞显示出CD184和CD195更高的表面受体和mRNA表达。表达阵列揭示了基因上调的差异,特别是对于细胞因子信号转导(SOCS)基因家族的抑制物,它们在细胞生长和调节中的JAK2 / STAT3信号转导和细胞骨髓细胞增生癌基因(c-MYC)中起作用。结论:LADR细胞如此独特,因为它们显示出较慢的增殖速率,更先进的发育,增加了FcεRI/ CD117和类胰蛋白酶的表达,具有不同的基因表达谱,并显示出对HIV-BAL,LAV,与LAD2细胞相比,TYBE和TYBE。因此,这种新细胞系是先前描述的少数FcεRI+人肥大细胞系的宝贵补充,可用于科学探索。

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