Establishing Primary and Stable Cell Lines from Frozen Wing Biopsies for Cellular, Physiological, and Genetic Studies in Bats
Fengyan Deng, Pedro Morales-Sosa, Andrea Bernal-Rivera, Yan Wang, Dai Tsuchiya, Jose Emmanuel Javier, Nicolas Rohner, Chongbei Zhao, Jasmin Camacho
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引用次数: 0
Abstract
Bats stand out among mammalian species for their exceptional traits, including the capacity to navigate through flight and echolocation, conserve energy through torpor/hibernation, harbor a multitude of viruses, exhibit resistance to disease, survive harsh environmental conditions, and demonstrate exceptional longevity compared to other mammals of similar size. In vivo studies of bats are challenging for several reasons, such as difficulty in locating and capturing them in their natural environments, limited accessibility, low sample size, environmental variation, long lifespans, slow reproductive rates, zoonotic disease risks, species protection, and ethical concerns. Thus, establishing alternative laboratory models is crucial for investigating the diverse physiological adaptations observed in bats. Obtaining quality cells from tissues is a critical first step for successful primary cell derivation. However, it is often impractical to collect fresh tissue and process the samples immediately for cell culture due to the resources required for isolating and expanding cells. As a result, frozen tissue is typically the starting resource for bat primary cell derivation, but cells in frozen tissue are usually damaged and have low integrity and viability. Isolating primary cells from frozen tissues thus poses a significant challenge. Herein, we present a successfully developed protocol for isolating primary dermal fibroblasts from frozen bat wing biopsies. This protocol marks a significant milestone, as this is the first protocol specifically focused on fibroblast isolation from bat frozen tissue. We also describe methods for primary cell characterization, genetic manipulation of primary cells through lentivirus transduction, and the development of stable cell lines. © 2024 Wiley Periodicals LLC.
Basic Protocol 1: Bat wing biopsy collection and preservation
Support Protocol 1: Blood collection from bat venipuncture
Basic Protocol 2: Isolation of primary fibroblasts from adult bat frozen wing biopsy
Support Protocol 2: Primary fibroblast culture and subculture
Support Protocol 3: Determination of growth curve and doubling time
Support Protocol 4: Cell banking and thawing of primary fibroblasts
Basic Protocol 3: Lentiviral transduction of bat primary fibroblasts
Basic Protocol 4: Bat stable fibroblast cell line development
Support Protocol 5: Bat fibroblast validation by immunofluorescence staining
Basic Protocol 5: Chromosome counting
从冷冻的蝙蝠翅膀活检组织中建立原始稳定的细胞系,用于蝙蝠的细胞、生理和遗传研究。
在哺乳动物中,蝙蝠以其特殊的性状脱颖而出,包括通过飞行和回声定位导航的能力、通过冬眠/休眠保存能量的能力、携带多种病毒的能力、对疾病的抵抗力、在恶劣环境条件下生存的能力,以及与其他体型相似的哺乳动物相比表现出的超长寿命。对蝙蝠进行活体研究具有挑战性,原因有很多,如在自然环境中寻找和捕捉蝙蝠的难度、可及性有限、样本量少、环境变化、寿命长、繁殖率慢、人畜共患病风险、物种保护和伦理问题等。因此,建立替代实验室模型对于研究蝙蝠的各种生理适应性至关重要。从组织中获取优质细胞是成功衍生原代细胞的关键第一步。然而,由于分离和扩增细胞需要大量资源,收集新鲜组织并立即处理样本进行细胞培养往往不切实际。因此,冷冻组织通常是蝙蝠原代细胞衍生的起始资源,但冷冻组织中的细胞通常已损坏,完整性和活力较低。因此,从冷冻组织中分离原代细胞是一项重大挑战。在本文中,我们介绍了一种成功开发的从冷冻蝙蝠翅膀活检组织中分离真皮原代成纤维细胞的方案。这是第一个专门从蝙蝠冷冻组织中分离成纤维细胞的方案,因此具有重要的里程碑意义。我们还介绍了原代细胞表征、通过慢病毒转导对原代细胞进行遗传操作以及开发稳定细胞系的方法。© 2024 Wiley Periodicals LLC.基本方案 1:采集和保存蝙蝠翅膀活检样本 支持方案 1:蝙蝠静脉穿刺采血 基本方案 2:从成年蝙蝠冷冻翅膀活检样本中分离原代成纤维细胞 支持方案 2:原代成纤维细胞的培养和亚培养 支持方案 3:确定生长曲线和倍增时间 支持方案 4:细胞储存和解冻原代成纤维细胞细胞库和解冻原代成纤维细胞 基本方案 3:慢病毒转导蝙蝠原代成纤维细胞 基本方案 4:蝙蝠稳定成纤维细胞系的开发 支持方案 5:通过免疫荧光染色验证蝙蝠成纤维细胞 基本方案 5:染色体计数。
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