Impact of platelet activation on the release of cell-free mitochondria and circulating mitochondrial DNA

被引:2
|
作者
Roch, Benoit [1 ,2 ]
Pisareva, Ekaterina [1 ]
Mirandola, Alexia [1 ]
Sanchez, Cynthia [1 ]
Pastor, Brice [1 ]
Tanos, Rita [1 ]
Frayssinoux, Florence [1 ]
Diab-Assaf, Mona [3 ]
Anker, Philippe [1 ]
Dache, Zahra Al Amir [1 ,4 ]
Thierry, Alain R. [1 ,4 ,5 ]
机构
[1] Montpellier Univ, IRCM Montpellier Canc Res Inst, INSERM U1194, F-34298 Montpellier, France
[2] Univ Hosp Montpellier, Arnaud De Villeneuve Hosp, Thorac Oncol Unit, F-34295 Montpellier, France
[3] Lebanese Univ Fanar, Fac Sci 2, Beirut, Lebanon
[4] ICM Inst Reg Canc Montpellier, F-34298 Montpellier, France
[5] IRCM Montpellier Canc Res Inst, 208 Ave Apothicaires,Parc Euromed, F-34298 Montpellier 5, France
关键词
Platelet; Mitochondria; circulating DNA; Circulating mitochondria; Quantitative PCR; Plasma; EXTRACELLULAR VESICLES; STRANDED-DNA; COPY NUMBER; BLOOD; QUANTIFICATION; MTDNA; MUTATION; PLASMA; FETAL; SIZE;
D O I
10.1016/j.cca.2023.117711
中图分类号
R446 [实验室诊断]; R-33 [实验医学、医学实验];
学科分类号
1001 ;
摘要
Background: Research on circulating mitochondrial DNA (cir-mtDNA) based diagnostic is insufficient, as to its function, origin, structural features, and particularly its standardization of isolation. To date, plasma preparation performed in previous studies do not take into consideration the potential bias resulting from the release of mitochondria by activated platelets.Methods: To tackle this, we compared the mtDNA amount determined by a standard plasma preparation method or a method optimally avoiding platelet activation. MtDNA extracted from the plasma of seven healthy individuals was quantified by Q-PCR in the course of the process of both methods submitted to filtration, freezing or differential centrifugation.Results: 98.7 to 99.4% of plasma mtDNA corresponded to extracellular mitochondria, either free or into large extracellular vesicles. Without platelet activation, the proportion of both types of entities remained preponderant (76-80%), but the amount of detected mtDNA decreased 67-fold.Conclusion: We show the high capacity of platelets to release free mitochondria in "in vitro" conditions. This represents a potent confounding factor when extracting mtDNA for cir-mtDNA investigation. Platelet activation during pre-analytical conditions should therefore be avoided when studying cir-mtDNA. Our findings lead to a profound revision of the assumptions previously made by most works in this field. Overall, our data suggest the need to characterize or isolate mtDNA associated various structural forms, as well as to standardize plasma preparation, to better circumscribe cir-mtDNA's diagnostic capacity.
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页数:8
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