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Plate-based Large-scale Cultivation of Caenorhabditis elegans: Sample Preparation for the Study of Metabolic Alterations in Diabetes

机译:板式大规模秀丽隐杆线虫的培养:糖尿病的代谢变化研究的样品制备。

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摘要

Culturing Caenorhabditis elegans (C. elegans) in a large-scale manner on agar plates can be time-consuming and difficult. This protocol describes a simple and inexpensive method to obtain a large number of animals for the isolation of proteins to proceed with a western blot, mass spectrometry, or further proteomics analyses. Furthermore, an increase of nematode numbers for immunostainings and the integration of multiple analyses under the same culturing conditions can easily be achieved. Additionally, a transfer between plates with different experimental conditions is facilitated. Common techniques in plate culture involve the transfer of a single C. elegans using a platinum wire and the transfer of populated agar chunks using a scalpel. However, with increasing nematode numbers, these techniques become overly time-consuming. This protocol describes the large-scale culture of C. elegans including numerous steps to minimize the impact of the sample preparation on the physiology of the worm. Fluid and shear stress can alter the lifespan of and metabolic processes in C. elegans, thus requiring a detailed description of the critical steps in order to retrieve reliable and reproducible results. C. elegans is a model organism, consisting of neuronal cells for up to one-third, but lacking blood vessels, thus providing the possibility to investigate solely neuronal alterations independent of vascular control. Recently, early neurodegeneration in diabetic retinopathy was found prior to vascular alterations. Thus, C. elegans is of special interest for studying general mechanisms of diabetic complications. For example, an increased formation of advanced glycation end products (AGEs) and reactive oxygen species (ROS) is observed, which are reproducibly found in C. elegans. Protocols to handle samples of adequate size for a broader spectrum of investigations are presented here, exemplified by the study of diabetes-induced biochemical alterations. In general, this protocol can be useful for studies requiring large C. elegans numbers and in which liquid culture is not suitable.
机译:在琼脂平板上大规模培养秀丽隐杆线虫(C. elegans)可能既费时又困难。该方案描述了一种简单且廉价的方法,可用于获取大量动物以分离蛋白质,以进行蛋白质印迹,质谱或进一步的蛋白质组学分析。此外,可以容易地实现用于免疫染色的线虫数量的增加以及在相同培养条件下的多种分析的整合。另外,促进了具有不同实验条件的板之间的转移。平板培养中的常用技术包括使用铂丝转移单个秀丽隐杆线虫和使用手术刀转移居住的琼脂块。但是,随着线虫数量的增加,这些技术变得非常耗时。该协议描述了秀丽隐杆线虫的大规模培养,包括许多步骤以最大程度地减少样品制备对蠕虫生理的影响。流体应力和剪切应力会改变秀丽隐杆线虫的寿命和新陈代谢过程,因此需要对关键步骤进行详细描述,以获取可靠且可重复的结果。秀丽隐杆线虫是一种模型生物,由多达三分之一但没有血管的神经元细胞组成,因此提供了独立于血管控制而仅调查神经元改变的可能性。最近,在糖尿病性血管病变之前发现了糖尿病性视网膜病变的早期神经变性。因此,秀丽隐杆线虫对于研究糖尿病并发症的一般机制特别感兴趣。例如,观察到先进的糖基化终产物(AGEs)和活性氧(ROS)的形成增加,可在秀丽隐杆线虫中发现。此处介绍了处理足够大小的样本以进行更广泛研究的方案,以糖尿病诱导的生化改变的研究为例。通常,此协议可用于需要大量秀丽隐杆线虫的研究,并且其中液体培养不适合。

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