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纯化的酶可改善成年胸腺上皮细胞的分离和鉴定。

Purified enzymes improve isolation and characterization of the adult thymic epithelium.

机构信息

Monash Immunology and Stem Cell Laboratories, Level 3, STRIP-1, Building 75, Monash University, Wellington Rd. Clayton, Victoria 3800, Australia.

出版信息

J Immunol Methods. 2012 Nov 30;385(1-2):23-34. doi: 10.1016/j.jim.2012.07.023. Epub 2012 Aug 11.

Abstract

The reproducible isolation and accurate characterization of thymic epithelial cell (TEC) subsets is of critical importance to the ongoing study of thymopoiesis and its functional decline with age. The study of adult TEC, however, is significantly hampered due to the severely low stromal to hematopoietic cell ratio. Non-biased digestion and enrichment protocols are thus essential to ensure optimal cell yield and accurate representation of stromal subsets, as close as possible to their in vivo representation. Current digestion protocols predominantly involve diverse, relatively impure enzymatic variants of crude collagenase and collagenase/dispase (col/disp) preparations, which have variable efficacy and are often suboptimal in their ability to mediate complete digestion of thymus tissue. To address these issues we compared traditional col/disp preparations with the latest panel of Liberase products that contain a blend of highly purified collagenase and neutral protease enzymes. Liberase enzymes revealed a more rapid, complete dissociation of thymus tissue; minimizing loss of viability and increasing recovery of thymic stromal cell (TSC) elements. In particular, the recovery and viability of TEC, notably the rare cortical subsets, were significantly enhanced with Liberase products containing medium to high levels of thermolysin. The improved stromal dissociation led to numerically increased TEC yield and total TEC RNA isolated from pooled digests of adult thymus. Furthermore, the increased recovery of TEC enhanced resolution and quantification of TEC subsets in both adult and aged mice, facilitating flow cytometric analysis on a per thymus basis. We further refined the adult TEC phenotype by correlating surface expression of known TEC markers, with expression of intracellular epithelial lineage markers, Keratin 5 and Keratin 8. The data reveal more extensive expression of K8 than previously recognized and indicates considerable heterogeneity still exists within currently defined adult TEC subsets.

摘要

胸腺上皮细胞 (TEC) 亚群的可再现分离和精确表征对于正在进行的胸腺发生研究及其随年龄的功能衰退至关重要。然而,由于基质与造血细胞的比例严重偏低,成人 TEC 的研究受到严重阻碍。因此,非偏见性的消化和富集方案对于确保最佳的细胞产量和基质亚群的准确表示至关重要,尽可能接近其体内表示。目前的消化方案主要涉及各种相对不纯的粗胶原酶和胶原酶/分散酶 (col/disp) 制剂的酶变体,这些变体的效果不同,并且在介导胸腺组织的完全消化方面往往不是最佳的。为了解决这些问题,我们将传统的 col/disp 制剂与最新的 Liberase 产品进行了比较,这些产品包含高度纯化的胶原酶和中性蛋白酶混合物。Liberase 酶显示出更快、更完全地分离胸腺组织;最大限度地减少活力损失并增加胸腺基质细胞 (TSC) 元素的回收。特别是,含有中等到高水平耐热素的 Liberase 产品显著增强了 TEC 的恢复和活力,特别是罕见的皮质亚群。基质解离的改善导致从成人胸腺的混合消化物中分离出的 TEC 产量和总 TEC RNA 的数值增加。此外,TEC 的高回收率增强了成年和老年小鼠中 TEC 亚群的分辨率和定量,从而促进了基于每个胸腺的流式细胞分析。我们通过将已知的 TEC 标志物的表面表达与细胞内上皮谱系标志物角蛋白 5 (K5) 和角蛋白 8 (K8) 的表达相关联,进一步细化了成人 TEC 表型。数据显示 K8 的表达比以前认识到的更广泛,并表明在当前定义的成人 TEC 亚群中仍然存在相当大的异质性。

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