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可蚀热熔胶水凝胶用于脊髓局部线粒体移植。

Erodible thermogelling hydrogels for localized mitochondrial transplantation to the spinal cord.

机构信息

University of Kentucky, Spinal Cord & Brain Injury Research Center, United States of America; Departments of Physiology & Neuroscience, College of Medicine, Lexington, KY 40536-0509, United States of America.

College of Engineering, Lexington, KY 40506, United States of America.

出版信息

Mitochondrion. 2022 May;64:145-155. doi: 10.1016/j.mito.2022.04.002. Epub 2022 Apr 6.

Abstract

We developed a thermal-gelling, erodible hydrogel system for localized delivery of viable mitochondria in vivo, as well as labeled transplanted mitochondria with specific dyes and/or genetically modified mitochondria tagged with red fluorescence protein (RFP). We also employed cell lines to optimize a hydrogel composed of methylcellulose and hyaluronic acid designed to preserve bioenergetics while facilitating mitochondrial release. We further investigated how transplantation of allogeneic or xenogeneic mitochondria into respective cell lines affects host cellular metabolism, as measured by MTS assay. We found that 70% of mitochondria are released from the hydrogel within 20 min at 37 °C, that the respiratory capacity of hydrogel-released mitochondria over 60 min was greater than those without gel, and that MTR-labeling of mitochondria is not indelible. RFP-tagged transgenic mitochondria isolated from modified SH-SY5Y human neuroblastoma cells showed effective uptake into both naïve SH-SY5Y cells and rat PC-12 cells, notably when released from hydrogel. The hydrogel both protected the mitochondria at physiological conditions in vitro while solidifying and diffusing within 60 min locally in situ. To assess metabolic effects, both cell lines were transplanted with different concentrations of SH-SY5Y or PC-12 cell line-derived mitochondria and all resulted in significant increases in metabolism at 6- and 24-hour after transplantation. Alternatively, transplanted mitochondria at highest concentration from rat brain and spinal cord tissues reduced metabolic activities after 24-hour. Along with hydrogel refinements, we are further investigating whether such metabolic changes are due to alterations in cell proliferation or the number of exogenous mitochondria incorporated into individual host cells.

摘要

我们开发了一种热凝胶、可侵蚀的水凝胶系统,用于在体内局部递送电镜下可见的活线粒体,以及用特定染料和/或带有红色荧光蛋白 (RFP) 的基因修饰线粒体标记移植的线粒体。我们还采用细胞系来优化由甲基纤维素和透明质酸组成的水凝胶,该水凝胶旨在保持生物能量的同时促进线粒体的释放。我们进一步研究了同种异体或异种异体线粒体移植到相应细胞系如何影响宿主细胞代谢,方法是通过 MTS 测定法进行测量。我们发现,70%的线粒体在 37°C 下 20 分钟内从水凝胶中释放出来,凝胶释放的线粒体在 60 分钟内的呼吸能力大于没有凝胶的线粒体,并且线粒体的 MTR 标记是不可擦除的。从修饰的 SH-SY5Y 人神经母细胞瘤细胞中分离出的带有 RFP 标记的转基因线粒体显示出有效进入未成熟的 SH-SY5Y 细胞和大鼠 PC-12 细胞的能力,尤其是从水凝胶中释放出来时。水凝胶在体外生理条件下既保护线粒体,又在 60 分钟内在局部原位固化和扩散。为了评估代谢效应,将不同浓度的 SH-SY5Y 或 PC-12 细胞系衍生的线粒体移植到两种细胞系中,结果均导致移植后 6 小时和 24 小时代谢显著增加。相反,来自大鼠脑和脊髓组织的最高浓度的移植线粒体在 24 小时后降低了代谢活性。随着水凝胶的改进,我们正在进一步研究这些代谢变化是否是由于细胞增殖的改变或单个宿主细胞中掺入的外源性线粒体数量的改变引起的。

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Mitochondrial transplantation for organ rescue.用于器官挽救的线粒体移植
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