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血小板浓缩物在储存 5 天期间活性氧生成和游离线粒体 DNA 的评估。

The evaluation of reactive oxygen species generation and free mitochondrial DNA in platelet concentrates during 5 days of storage.

机构信息

Blood Transfusion Research Center, High Institute for Research and Education in Transfusion Medicine, Tehran, Iran.

出版信息

Blood Coagul Fibrinolysis. 2023 Mar 1;34(2):105-110. doi: 10.1097/MBC.0000000000001187. Epub 2022 Dec 22.

Abstract

Oxidative stress and mitochondrial damage are causes of platelet storage lesions (PSLs). Mitochondrial damage causes mitochondrial DNA (mtDNA) to be released into the extracellular space. MtDNA in platelet concentrates is considered damage-associated molecular patterns (DAMPs) and is one of the major causes of PSLs. The mechanism of mtDNA release in platelet concentrates has not been thoroughly investigated. This study aimed to determine the effect of reactive oxygen species (ROS) on mtDNA release in platelet concentrates during storage. Ten platelet concentrates from healthy donors were obtained in this investigation. Platelet concentrates were prepared by platelet-rich plasma (PRP) and stored at 22 ± 2 C° with gentle agitation. Platelet concentrates were subjected to flow cytometry and real-time PCR to evaluate total ROS and free mtDNA on days 0, 3, and 5 of platelet concentrate storage. Total ROS detected significantly increased from day 0 to day 5 of platelet concentrate storage (P = 0.0079). The mean of copy numbers of free mtDNA on day 0 increased from 3.43 × 106 ± 1.57 × 106 to 2.85 × 107 ± 1.51 × 107 (molecules/μl) on the fifth day of platelet concentrate storage, and it was statistically significant (P = 0.0039). In addition, LDH enzyme activity significantly increased during platelet concentrate storage (P < 0.0001). Also, releasing mtDNA in platelet concentrates was directly correlated with total ROS generation (P = 0.021, r = 0.61) and LDH activity (P = 0.04, r = 0.44). The evidence from this study confirmed the increasing level mtDNA copy numbers in platelet concentrates during storage, and the amount of free mtDNA is directly correlated with ROS generation and platelet lysis during 5 days of platelet concentrate storage. Finally, these changes may be related to DAMPs in the platelet concentrates.

摘要

氧化应激和线粒体损伤是血小板储存损伤(PSL)的原因。线粒体损伤导致线粒体 DNA(mtDNA)释放到细胞外空间。血小板浓缩物中的 mtDNA 被认为是损伤相关分子模式(DAMP),是 PSL 的主要原因之一。mtDNA 在血小板浓缩物中的释放机制尚未得到彻底研究。本研究旨在确定在储存过程中活性氧(ROS)对血小板浓缩物中 mtDNA 释放的影响。本研究共获得 10 份来自健康供体的血小板浓缩物。通过富含血小板的血浆(PRP)制备血小板浓缩物,并在 22±2°C 温和搅拌下储存。在血小板浓缩物储存的第 0、3 和 5 天,通过流式细胞术和实时 PCR 评估总 ROS 和游离 mtDNA。从血小板浓缩物储存的第 0 天到第 5 天,总 ROS 检测值显著增加(P=0.0079)。第 0 天游离 mtDNA 的平均拷贝数从 3.43×106±1.57×106增加到第 5 天的 2.85×107±1.51×107(分子/μl),差异具有统计学意义(P=0.0039)。此外,在血小板浓缩物储存过程中 LDH 酶活性显著增加(P<0.0001)。另外,血小板浓缩物中 mtDNA 的释放与总 ROS 生成直接相关(P=0.021,r=0.61)和 LDH 活性(P=0.04,r=0.44)。本研究的证据证实了储存过程中血小板浓缩物中 mtDNA 拷贝数的增加水平,并且游离 mtDNA 的量与 5 天血小板浓缩物储存过程中的 ROS 生成和血小板溶解直接相关。最后,这些变化可能与血小板浓缩物中的 DAMPs 有关。

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