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[淋巴瘤免疫分型] 胰酶消化制备样品,对细胞的表型什么的有影响吗

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发表于 2013-10-28 15:07:46 | 显示全部楼层 |阅读模式
到底胰酶等制备方法对细胞表型和功能有没有影响
正方观点 (4)

我看书上的新鲜实体组织的样品制备第一个就写的就是胰酶消化法,因此可以用于流式样本处理。

VS
反方观点 (1)

既然是酶,肯定对样品表面的标记有影响,当然也有可能影响功能

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    组织样本处理不好?流式中文网原研的魔滤®魔杵®套装,低成本解决,高质量收获
    发表于 2013-10-30 22:11:51 | 显示全部楼层
    这个投票的两个观点其实应该综合到一起,而不应该是对立的。
    应该说,胰酶消化对样本制备出的单细胞悬液活性有影响,从而影响到表面标记的表达,但是胰酶消化的标本是可以用在流式细胞术检测上的,否则你说贴壁细胞怎么做流式?物理方法?物理方法损伤更大。
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    发表于 2013-11-1 11:33:37 | 显示全部楼层

    不是这个意思,而是由于胰酶对细胞的损伤,导致较多细胞死亡或细胞膜受损,故容易出现非特异性染色。不过可以通过死活细胞鉴别试剂或PI染料,可以将这些细胞排除掉,剩余的活细胞分析还是跟其它正常情况一样的。
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    发表于 2013-11-1 16:30:06 来自手机 | 显示全部楼层
    20071271 发表于 2013-11-01 11:57:27


    就是说,其实胰酶不会对细胞表面标记产生影响,对吧

    是的,但是前提是要排除死细胞和碎片,否则这些细胞的非特异性染色会影响分析。
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    发表于 2013-11-4 18:53:23 | 显示全部楼层
    dragonhzqsmmu 发表于 2013-11-4 14:54
    个人感觉只要是酶消化都会对表面标志有所影响,只不过随着选择的酶的种类、消化时间、温度等条件的影响对待 ...

    感谢@dragonhzqsmmu 站友的分享,确实跟酶有些关系。我将该文中的相关章节摘录如下:

    To separate individual cells from the plaques, we first used various collagenases that were first tested on PBMCs for preserving the cell surface markers CD3, CD4, CD16, CD45, CD45RA, CD197, CD28, CD27, HLA-DR, and CD38(研究了不同胶原酶对这些标记的影响).
    We treated PBMCs with collagenase XIs(这个酶影响较大) diluted at 5, 10, and 2.5 mg/mL. The lowest enzyme concentration resulted in the reduction of CD8 expression by 90% compared with nontreated cells. Also, the expression of CD4, CD3, CD27, and CD28 was reduced by 40%, 12%, 50%, and 42%, respectively. Because of these strong effects, the ability of this enzyme to liberate cells was not studied further.
    Second, we treated PBMCs with collagenase IV at 10, 5, and 2.5 mg/mL and noticed that at the highest concentrations, the expression of CD4 and CD8 were reduced by 29% and 23%, respectively. At 1.25 mg/mL collagenase IV, the surface markers expression was decreased by 4.9±3.4% compared with that on untreated PBMCs. Third, we treated cells with Liberase DL. At the concentrations of 62.5 and 31.5 μg/mL, CD4 was reduced by ≈70%, whereas at 15 μg/mL, the expression of this marker was reduced by only 20±7%. The expression levels of CD3, CD8, CD16, CD45, and HLA-DR were affected marginally.
    To liberate cells from atherosclerotic plaques, we applied enzymes at concentrations that did not grossly decrease expression of cell surface molecules in PBMCs. Freshly excised plaques were digested with collagenase IV (2.5 and 1.25 mg/mL) and Liberase DL (25 and 12.5 μg/mL) in the presence of 0.2 mg/mL DNase I for 1 hour at 37°C. The cells were then stained with monoclonal antibodies for CD45, CD3, CD4, and CD8. Collagenase IV at 1.25 mg/mL liberated more lymphocytes than did digestion with 2.5 mg/mL as evaluated by the relative amount of lymphocytes in the gate defined on side scatter (SSC) versus CD45 expression.
    On the basis of the relative lymphocyte (CD45+) yield, we chose treatment with collagenase IV for 1 hour at 37°C(这是最后选择的最佳 条件) as an efficient method to liberate lymphocytes from atherosclerotic plaques while largely preserving cell surface markers. We used this protocol in all our subsequent experiments described below. However, the concentration of the enzyme has to be adjusted for each enzyme batch and in our experiments varied between 1 and 1.25 mg/mL.
    组织样本处理不好?流式中文网原研的魔滤®魔杵®套装,低成本解决,高质量收获
    发表于 2013-11-5 09:50:01 | 显示全部楼层
    20071271 发表于 2013-11-5 09:47
    但又不能不用胰酶消化,怎么办呢,特别是染色都比较dim的情况下,如何是好 ...

    别纠结了,做吧。各种实体组织细胞的文章都这么做下来的
    组织样本处理不好?流式中文网原研的魔滤®魔杵®套装,低成本解决,高质量收获
    发表于 2013-11-5 09:53:42 | 显示全部楼层
    20071271 发表于 2013-11-5 09:51
    那胰酶的影响有多大呢

    至少在我帮研究生做的那些实验中,没注意到。只需排除死细胞即可。

    上面这篇文章,我觉得一方面他们研究的是胶原酶的影响,另一方面研究的是淋巴细胞标记,这两方面跟你的实验都没关系。所以无需过分担心。排除死细胞才是关键所在。
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    发表于 2013-11-7 11:36:21 | 显示全部楼层
    dragonhzqsmmu 发表于 2013-11-7 11:31
    给个建议,不知道对不对,试试美天旎的组织粉碎仪器,记得BD公司也有类似的产品,好像基本上依赖物理作用, ...

    组织研磨器是只针对组织团块,对于培养的贴壁细胞还是只能用胰酶消化了。

    我们平时在临床上都是用BD的medimachine研磨组织块,发现得率不高,所以如果要做,需尽可能获得比较多的组织。
    流式中文网FlowGuard®流式专用保存液,无需冻存,稳定保护各类流式样本,从容完成实验
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