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一种用于研究神经突生长对牙髓旁分泌信号反应的共培养方法。

A Co-Culture Method to Study Neurite Outgrowth in Response to Dental Pulp Paracrine Signals.

作者信息

Barkley Courtney, Serra Rosa, Peters Sarah B

机构信息

Cell, Developmental and Integrative Biology Department, University of Alabama at Birmingham.

Cell, Developmental and Integrative Biology Department, University of Alabama at Birmingham;

出版信息

J Vis Exp. 2020 Feb 14(156). doi: 10.3791/60809.

Abstract

Tooth innervation allows teeth to sense pressure, temperature and inflammation, all of which are crucial to the use and maintenance of the tooth organ. Without sensory innervation, daily oral activities would cause irreparable damage. Despite its importance, the roles of innervation in tooth development and maintenance have been largely overlooked. Several studies have demonstrated that DP cells secrete extracellular matrix proteins and paracrine signals to attract and guide TG axons into and throughout the tooth. However, few studies have provided detailed insight into the crosstalk between the DP mesenchyme and neuronal afferents. To address this gap in knowledge, researchers have begun to utilize co-cultures and a variety of techniques to investigate these interactions. Here, we demonstrate the multiple steps involved in co-culturing primary DP cells with TG neurons dispersed on an overlying transwell filter with large diameter pores to allow axonal growth through the pores. Primary DP cells with the gene of interest flanked by loxP sites were utilized to facilitate gene deletion using an Adenovirus-Cre-GFP recombinase system. Using TG neurons from the Thy1-YFP mouse allowed for precise afferent imaging, with expression well above background levels by confocal microscopy. The DP responses can be investigated via protein or RNA collection and analysis, or alternatively, through immunofluorescent staining of DP cells plated on removable glass coverslips. Media can be analyzed using techniques such as proteomic analyses, although this will require albumin depletion due to the presence of fetal bovine serum in the media. This protocol provides a simple method that can be manipulated to study the morphological, genetic, and cytoskeletal responses of TG neurons and DP cells in response to the controlled environment of a co-culture assay.

摘要

牙齿的神经支配使牙齿能够感知压力、温度和炎症,所有这些对于牙齿器官的使用和维持都至关重要。没有感觉神经支配,日常口腔活动将造成无法弥补的损害。尽管其很重要,但神经支配在牙齿发育和维持中的作用在很大程度上被忽视了。几项研究表明,牙髓乳头(DP)细胞分泌细胞外基质蛋白和旁分泌信号,以吸引并引导三叉神经节(TG)轴突进入并贯穿牙齿。然而,很少有研究深入探讨DP间充质与神经传入之间的相互作用。为了填补这一知识空白,研究人员已开始利用共培养和各种技术来研究这些相互作用。在此,我们展示了将原代DP细胞与分散在上层大孔径跨膜滤器上的TG神经元进行共培养所涉及的多个步骤,以允许轴突通过这些孔生长。利用loxP位点侧翼带有感兴趣基因的原代DP细胞,通过腺病毒-Cre-GFP重组酶系统促进基因缺失。使用来自Thy1-YFP小鼠的TG神经元可实现精确的传入成像,通过共聚焦显微镜观察,其表达远高于背景水平。DP反应可通过蛋白质或RNA的收集与分析来研究,或者通过对铺在可移除玻璃盖玻片上的DP细胞进行免疫荧光染色来研究。尽管由于培养基中存在胎牛血清,这需要去除白蛋白,但培养基可以使用蛋白质组学分析等技术进行分析。该方案提供了一种简单的方法,可加以调整以研究TG神经元和DP细胞在共培养试验的可控环境下的形态、遗传和细胞骨架反应。

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