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从小鼠中分离和培养原代周细胞。

Isolation and Culture of Primary Pericytes from Mouse.

作者信息

McErlain Tamara, Branco Cristina M, Murgai Meera

机构信息

Laboratory of Cancer Biology and Genetics, National Cancer Institute, National Institutes of Health, Bethesda, MD, USA.

Patrick G. Johnston Centre for Cancer Research, Queen's University Belfast, Belfast, UK.

出版信息

Bio Protoc. 2025 Apr 20;15(8):e5288. doi: 10.21769/BioProtoc.5288.

Abstract

Pericytes are essential for tissue homeostasis, functioning to regulate capillary blood flow. Dysfunctional pericytes are implicated in various pathologies, including cancer progression. Despite their important function in both health and disease, pericytes remain understudied due to a lack of robust model systems that accurately reflect their in vivo biology. Here, we present a comprehensive protocol for isolating and culturing primary pericytes from murine lung, brain, bone, and liver tissues, based on NG2 expression using an antibody-conjugated magnetic bead approach. Our protocol emphasizes the importance of physiological oxygen tension during ex vivo culture (10% O for lung pericytes and 5% O for brain, bone, and liver pericytes). These conditions stabilize the expression of characteristic pericyte markers at both the transcriptional and protein levels. Importantly, we optimized growth conditions to limit the expression of the plasticity factor in order to prevent spontaneous phenotypic switching in vitro. This protocol provides a reliable and reproducible method for obtaining pericytes suitable for high-throughput analyses in order to explore pericyte biology in both physiological and pathological contexts. Key features • Isolation of primary pericytes from mouse lung, brain, bone, and liver. • Emphasis on physioxic culturing conditions to better maintain pericyte phenotype. • Representative of pericyte biology in both health and disease contexts.

摘要

周细胞对于组织稳态至关重要,其功能是调节毛细血管血流。功能失调的周细胞与包括癌症进展在内的各种病理状况有关。尽管周细胞在健康和疾病中都发挥着重要作用,但由于缺乏能准确反映其体内生物学特性的强大模型系统,周细胞仍未得到充分研究。在此,我们基于使用抗体偶联磁珠方法对NG2表达情况,提出了一种从鼠肺、脑、骨和肝组织中分离和培养原代周细胞的综合方案。我们的方案强调了体外培养过程中生理氧张力的重要性(肺周细胞为10%氧气,脑、骨和肝周细胞为5%氧气)。这些条件在转录和蛋白质水平上稳定了特征性周细胞标志物的表达。重要的是,我们优化了生长条件以限制可塑性因子的表达,从而防止体外自发的表型转换。该方案提供了一种可靠且可重复的方法来获取适合高通量分析的周细胞,以便在生理和病理背景下探索周细胞生物学。关键特性• 从小鼠肺、脑、骨和肝中分离原代周细胞。• 强调生理氧培养条件以更好地维持周细胞表型。• 代表健康和疾病背景下的周细胞生物学。

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