| Isolation of Microvascular Endothelial Cells
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Author:
Date:
2018-06-20
[Abstract] The vascular endothelium is essential to normal vascular homeostasis. Its dysfunction participates in various cardiovascular disorders. Murine endothelial cell culture is an important tool for cardiovascular disease research. This protocol demonstrates a quick, efficient method for the isolation of microvascular endothelial cells from murine tissues without any special equipment. To isolate endothelial cells, the lung or heart were mechanically minced and enzymatically digested with collagenase and trypsin. The single cell suspension obtained was then incubated with an anti-CD31, anti-CD105 antibody and with biotinylated isolectin B-4. The endothelial cells were harvested using magnetic bead separation with rat anti-mouse Ig- and streptavidin-conjugated microbeads. Endothelial cells were ...
[摘要] 血管内皮是正常血管稳态所必需的。其功能障碍参与各种心血管疾病。小鼠内皮细胞培养是心血管疾病研究的重要工具。该协议演示了一种快速,有效的方法从小鼠组织中分离微血管内皮细胞而无需任何特殊设备。为了分离内皮细胞,将肺或心脏机械切碎并用胶原酶和胰蛋白酶进行酶促消化。然后将获得的单细胞悬浮液与抗CD31,抗CD105抗体和生物素化的异凝集素B-4温育。使用大鼠抗小鼠Ig-和链霉亲和素缀合的微珠,使用磁珠分离收获内皮细胞。扩张内皮细胞并收集用于随后的分析。这些培养物的形态和表型特征在培养10代以上保持稳定。在任何阶段没有过度生长的非内皮来源的污染细胞。
【背景】微血管内皮细胞通过调节白细胞再循环和作为T淋巴细胞的抗原呈递细胞而在免疫应答的发展中起中心作用。内皮的良好状态对血管稳态很重要。功能失调的内皮参与各种心血管疾病,包括动脉粥样硬化,血管炎和缺血/再灌注损伤(Cid et al。,2004; Wang等人,2007)。因此,体外培养的内皮细胞培养物是研究血管生理学和疾病病理学的重要工具。然而,分离原代鼠类内皮细胞被认为是特别困难的,因为大多数描述的方案涉及用消化酶灌注器官或大血管和耗时的纯化过程(Gumkowski等人,1987) 。
该协议的目的是提供一种简单的方法,不需要使用任何特殊设备即可从肺/心脏中分离和扩展内皮细胞。使用这种方法,我们以前补充了体内研究,证明了CD31信号传导在内皮细胞细胞保护中的重要性(Cheung等人,2015年)。 ...
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| Isolation of Murine Alveolar Type II Epithelial Cells
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Author:
Date:
2017-05-20
[Abstract] We have optimized a protocol for isolation of alveolar type II epithelial cells from mouse lung. Lung cell suspensions are prepared by intratracheal instillation of dispase and agarose followed by mechanical disaggregation of the lungs. Alveolar type II epithelial cells are purified from these lung cell suspensions through magnetic-based negative selection using a Biotin-antibody, Streptavidin-MicroBeads system. The purified alveolar type II epithelial cells can be cultured and maintained on fibronectin-coated plates in DMEM with 10% FBS. This protocol enables specific investigation of alveolar type II epithelial cells at molecular and cellular levels and provides an important tool to investigate in vitro the mechanisms underlying lung pathogenesis.
[摘要] 我们优化了从小鼠肺分离肺泡II型上皮细胞的方案。通过气管内滴注分泌酶和琼脂糖,然后机械解聚肺来制备肺细胞悬浮液。通过使用生物素抗体Streptavidin-MicroBeads系统的磁性阴性选择,从这些肺细胞悬液中纯化肺泡II型上皮细胞。可以将纯化的肺泡II型上皮细胞培养并维持在含有10%FBS的DMEM中的纤连蛋白包被的平板上。该方案能够在分子和细胞水平上对肺泡II型上皮细胞进行特异性研究,并提供了一种重要的工具,用于在体外研究肺发病机制的机制。
背景 肺泡II型上皮细胞在肺泡完整性维持,表面活性蛋白合成和分泌中起关键作用,并防止细菌和病毒的肺部感染。最近使用小鼠肺癌模型的研究已经证明,肺泡II型上皮细胞是由化学致癌物质和致癌突变诱导的腺瘤/腺癌的关键细胞(Qu 等人,2015; Zhou > et al。,2015和2017)。为了进一步扩大我们对肺泡II型上皮细胞在体内肺发病机制中的作用的理解,需要分离肺泡II型上皮细胞以允许体外精确的机理分析, EM>。基于先前的研究(Corti等人,1996; Rice等人,2002),在我们的实验室中使用了一种修饰的方法来分离高度纯化的,可行的和可培养的来自小鼠的肺泡II型上皮细胞(Zhou等人,2015; Sun等人,2016)。
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| FACS-based Satellite Cell Isolation From Mouse Hind Limb Muscles
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Author:
Date:
2015-08-20
[Abstract] Fluorescence Activated Cell Sorting (FACS) is a sensitive and accurate method for purifying satellite cells, or muscle stem cells, from adult mouse skeletal muscle (Liu et al., 2013; Sacco et al., 2008; Tierney et al., 2014). Mechanical and enzymatic digestion of hind limb muscles releases mononuclear muscle cells into suspension. This protocol employs fractionation strategies to deplete cells expressing the cell surface markers CD45, CD31, CD11b and Ly-6A/E-Sca1, both by magnetic separation and FACS-based exclusion, and positively select for cells expressing a7-integrin and CD34. This enables the researcher to successfully enrich satellite cells that uniformly express the paired-box transcription factor Pax7 and are capable of long-term self-renewal, skeletal ...
[摘要] 荧光活化细胞分选(FACS)是用于从成年小鼠骨骼肌纯化卫星细胞或肌肉干细胞的灵敏和精确的方法(Liu等人,2013; Sacco等人, ,2008; Tierney ,,2014)。 后肢肌肉的机械和酶消化将单核肌细胞释放到悬浮液中。 该方案采用分级分离策略,通过磁性分离和基于FACS的排除,耗尽表达细胞表面标记CD45,CD31,CD11b和Ly-6A/E-Sca1的细胞,并阳性选择表达α7-整联蛋白和CD34的细胞。 这使得研究者能够成功地富集均匀表达配对盒转录因子Pax7并且能够长期自我更新,骨骼肌修复和肌肉干细胞池再增殖的卫星细胞。
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