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Divide-and-Conquer Matrisome Protein (DC-MaP) Strategy: An MS-Friendly Approach to Proteomic Matrisome Characterization

机译:分裂和征服矩阵蛋白(DC-MAP)策略:对蛋白质组学矩阵表征的MS友好方法

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摘要

Currently, the extracellular matrix (ECM) is considered a pivotal complex meshwork of macromolecules playing a plethora of biomolecular functions in health and disease beyond its commonly known mechanical role. Only by unraveling its composition can we leverage related tissue engineering and pharmacological efforts. Nevertheless, its unbiased proteomic identification still encounters some limitations mainly due to partial ECM enrichment by precipitation, sequential fractionation using unfriendly-mass spectrometry (MS) detergents, and resuspension with harsh reagents that need to be entirely removed prior to analysis. These methods can be technically challenging and labor-intensive, which affects the reproducibility of ECM identification and induces protein loss. Here, we present a simple new method applicable to tissue fragments of 10 mg and more. The technique has been validated on human ovarian tissue and involves a standardized procedure for sample processing with an MS-compatible detergent and combined centrifugation. This two-step protocol eliminates the need for laborious sample clarification and divides our samples into 2 fractions, soluble and insoluble, successively enriched with matrisome-associated (ECM-interacting) and core matrisome (structural ECM) proteins.
机译:目前,细胞外基质(ECM)被认为是在常规众所周知的机械作用的健康和疾病中占大重组的枢转复杂网状作用。只有通过解开其组合物,我们可以利用相关的组织工程和药理学努力。然而,其无偏念珠菌仍然遇到一些限制,主要是由于沉淀的部分ECM富集,使用不友好的质谱(MS)洗涤剂的顺序分馏,并用苛刻的试剂重新悬浮,在分析之前需要完全除去。这些方法可以在技术上具有挑战性和劳动密集型,影响ECM鉴定的再现性并诱导蛋白质损失。在这里,我们提出了一种简单的新方法,适用于10毫克和更多的组织片段。该技术已在人卵巢组织上验证,涉及用MS相容的洗涤剂和组合离心的样品加工的标准化程序。该两步方案消除了对少数份数,将样品分成2个级分,溶于和不溶性的需求,连续地富含母细胞组合(ECM相互作用)和核心矩阵(结构ECM)蛋白质。

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