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Establishment of preanalytical conditions for microRNA profile analysis of clinical plasma samples

The relationship between the expression of microRNAs (miRNAs) in blood and a variety of diseases has been investigated. MiRNA-based liquid biopsy has attracted much attention, and cancer-specific miRNAs have been reported. However, the results of analyses of the expression of these miRNAs vary among...

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Autores principales: Suzuki, Kuno, Yamaguchi, Tatsuya, Kohda, Masakazu, Tanaka, Masami, Takemura, Hiroyuki, Wakita, Mitsuru, Tabe, Yoko, Kato, Shunsuke, Nasu, Motomi, Hashimoto, Takashi, Mine, Shinji, Serizawa, Nobuko, Tomishima, Ko, Nagahara, Akihito, Matsuda, Takahisa, Yamaji, Taiki, Tsugane, Shoichiro, Saito, Yutaka, Daiko, Hiroyuki, Yoshikawa, Takaki, Kato, Ken, Okusaka, Takuji, Ochiya, Takahiro, Yamamoto, Yusuke, Yotsui, Shoji, Yamamoto, Takashi, Yamasaki, Tomoyuki, Miyata, Hiroshi, Yasui, Masayoshi, Omori, Takeshi, Ohkawa, Kazuyoshi, Ikezawa, Kenji, Nakabori, Tasuku, Sugimoto, Naotoshi, Kudo, Toshihiro, Yoshida, Keiichi, Ohue, Masayuki, Nishizawa, Takashi
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2022
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9750036/
https://www.ncbi.nlm.nih.gov/pubmed/36516194
http://dx.doi.org/10.1371/journal.pone.0278927
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author Suzuki, Kuno
Yamaguchi, Tatsuya
Kohda, Masakazu
Tanaka, Masami
Takemura, Hiroyuki
Wakita, Mitsuru
Tabe, Yoko
Kato, Shunsuke
Nasu, Motomi
Hashimoto, Takashi
Mine, Shinji
Serizawa, Nobuko
Tomishima, Ko
Nagahara, Akihito
Matsuda, Takahisa
Yamaji, Taiki
Tsugane, Shoichiro
Saito, Yutaka
Daiko, Hiroyuki
Yoshikawa, Takaki
Kato, Ken
Okusaka, Takuji
Ochiya, Takahiro
Yamamoto, Yusuke
Yotsui, Shoji
Yamamoto, Takashi
Yamasaki, Tomoyuki
Miyata, Hiroshi
Yasui, Masayoshi
Omori, Takeshi
Ohkawa, Kazuyoshi
Ikezawa, Kenji
Nakabori, Tasuku
Sugimoto, Naotoshi
Kudo, Toshihiro
Yoshida, Keiichi
Ohue, Masayuki
Nishizawa, Takashi
author_facet Suzuki, Kuno
Yamaguchi, Tatsuya
Kohda, Masakazu
Tanaka, Masami
Takemura, Hiroyuki
Wakita, Mitsuru
Tabe, Yoko
Kato, Shunsuke
Nasu, Motomi
Hashimoto, Takashi
Mine, Shinji
Serizawa, Nobuko
Tomishima, Ko
Nagahara, Akihito
Matsuda, Takahisa
Yamaji, Taiki
Tsugane, Shoichiro
Saito, Yutaka
Daiko, Hiroyuki
Yoshikawa, Takaki
Kato, Ken
Okusaka, Takuji
Ochiya, Takahiro
Yamamoto, Yusuke
Yotsui, Shoji
Yamamoto, Takashi
Yamasaki, Tomoyuki
Miyata, Hiroshi
Yasui, Masayoshi
Omori, Takeshi
Ohkawa, Kazuyoshi
Ikezawa, Kenji
Nakabori, Tasuku
Sugimoto, Naotoshi
Kudo, Toshihiro
Yoshida, Keiichi
Ohue, Masayuki
Nishizawa, Takashi
author_sort Suzuki, Kuno
collection PubMed
description The relationship between the expression of microRNAs (miRNAs) in blood and a variety of diseases has been investigated. MiRNA-based liquid biopsy has attracted much attention, and cancer-specific miRNAs have been reported. However, the results of analyses of the expression of these miRNAs vary among studies. The reproduction of results regarding miRNA expression levels could be difficult if there are differences in the data acquisition process. Previous studies have shown that the anticoagulant type used during plasma preparation and sample storage conditions could contribute to differences in measured miRNA levels. Thus, the impact of these preanalytical conditions on comprehensive miRNA expression profiles was examined. First, the miRNA expression profiles of samples obtained from healthy volunteers were analyzed using next-generation sequencing. Based on an analysis of the library concentration, human genome identification rate, ratio of unique sequences and expression profiles, the optimal preanalytical conditions for obtaining highly reproducible miRNA expression profiles were established. The optimal preanalytical conditions were as follows: ethylenediaminetetraacetic acid (EDTA) as the anticoagulant, whole-blood storage at room temperature within 6 hours, and plasma storage at 4°C or -20°C within 30 days. Next, plasma samples were collected from 60 cancer patients (3 facilities × 20 patients/facility), and miRNA expression profiles were analyzed. There were no significant differences in measurements except in the expression of erythrocyte-derived hsa-miR-451a. However, the variation in hsa-miR-451a levels was smaller among facilities than among individuals. This finding suggests that samples obtained from the same facility could show significantly different degrees of hemolysis across individuals. We found that the standardization of anticoagulant use and storage conditions contributed to reducing the variation in sample quality across facilities. The findings from this study could be useful in developing protocols for collecting samples from multiple facilities for cancer screening tests.
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spelling pubmed-97500362022-12-15 Establishment of preanalytical conditions for microRNA profile analysis of clinical plasma samples Suzuki, Kuno Yamaguchi, Tatsuya Kohda, Masakazu Tanaka, Masami Takemura, Hiroyuki Wakita, Mitsuru Tabe, Yoko Kato, Shunsuke Nasu, Motomi Hashimoto, Takashi Mine, Shinji Serizawa, Nobuko Tomishima, Ko Nagahara, Akihito Matsuda, Takahisa Yamaji, Taiki Tsugane, Shoichiro Saito, Yutaka Daiko, Hiroyuki Yoshikawa, Takaki Kato, Ken Okusaka, Takuji Ochiya, Takahiro Yamamoto, Yusuke Yotsui, Shoji Yamamoto, Takashi Yamasaki, Tomoyuki Miyata, Hiroshi Yasui, Masayoshi Omori, Takeshi Ohkawa, Kazuyoshi Ikezawa, Kenji Nakabori, Tasuku Sugimoto, Naotoshi Kudo, Toshihiro Yoshida, Keiichi Ohue, Masayuki Nishizawa, Takashi PLoS One Research Article The relationship between the expression of microRNAs (miRNAs) in blood and a variety of diseases has been investigated. MiRNA-based liquid biopsy has attracted much attention, and cancer-specific miRNAs have been reported. However, the results of analyses of the expression of these miRNAs vary among studies. The reproduction of results regarding miRNA expression levels could be difficult if there are differences in the data acquisition process. Previous studies have shown that the anticoagulant type used during plasma preparation and sample storage conditions could contribute to differences in measured miRNA levels. Thus, the impact of these preanalytical conditions on comprehensive miRNA expression profiles was examined. First, the miRNA expression profiles of samples obtained from healthy volunteers were analyzed using next-generation sequencing. Based on an analysis of the library concentration, human genome identification rate, ratio of unique sequences and expression profiles, the optimal preanalytical conditions for obtaining highly reproducible miRNA expression profiles were established. The optimal preanalytical conditions were as follows: ethylenediaminetetraacetic acid (EDTA) as the anticoagulant, whole-blood storage at room temperature within 6 hours, and plasma storage at 4°C or -20°C within 30 days. Next, plasma samples were collected from 60 cancer patients (3 facilities × 20 patients/facility), and miRNA expression profiles were analyzed. There were no significant differences in measurements except in the expression of erythrocyte-derived hsa-miR-451a. However, the variation in hsa-miR-451a levels was smaller among facilities than among individuals. This finding suggests that samples obtained from the same facility could show significantly different degrees of hemolysis across individuals. We found that the standardization of anticoagulant use and storage conditions contributed to reducing the variation in sample quality across facilities. The findings from this study could be useful in developing protocols for collecting samples from multiple facilities for cancer screening tests. Public Library of Science 2022-12-14 /pmc/articles/PMC9750036/ /pubmed/36516194 http://dx.doi.org/10.1371/journal.pone.0278927 Text en © 2022 Suzuki et al https://creativecommons.org/licenses/by/4.0/This is an open access article distributed under the terms of the Creative Commons Attribution License (https://creativecommons.org/licenses/by/4.0/) , which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
spellingShingle Research Article
Suzuki, Kuno
Yamaguchi, Tatsuya
Kohda, Masakazu
Tanaka, Masami
Takemura, Hiroyuki
Wakita, Mitsuru
Tabe, Yoko
Kato, Shunsuke
Nasu, Motomi
Hashimoto, Takashi
Mine, Shinji
Serizawa, Nobuko
Tomishima, Ko
Nagahara, Akihito
Matsuda, Takahisa
Yamaji, Taiki
Tsugane, Shoichiro
Saito, Yutaka
Daiko, Hiroyuki
Yoshikawa, Takaki
Kato, Ken
Okusaka, Takuji
Ochiya, Takahiro
Yamamoto, Yusuke
Yotsui, Shoji
Yamamoto, Takashi
Yamasaki, Tomoyuki
Miyata, Hiroshi
Yasui, Masayoshi
Omori, Takeshi
Ohkawa, Kazuyoshi
Ikezawa, Kenji
Nakabori, Tasuku
Sugimoto, Naotoshi
Kudo, Toshihiro
Yoshida, Keiichi
Ohue, Masayuki
Nishizawa, Takashi
Establishment of preanalytical conditions for microRNA profile analysis of clinical plasma samples
title Establishment of preanalytical conditions for microRNA profile analysis of clinical plasma samples
title_full Establishment of preanalytical conditions for microRNA profile analysis of clinical plasma samples
title_fullStr Establishment of preanalytical conditions for microRNA profile analysis of clinical plasma samples
title_full_unstemmed Establishment of preanalytical conditions for microRNA profile analysis of clinical plasma samples
title_short Establishment of preanalytical conditions for microRNA profile analysis of clinical plasma samples
title_sort establishment of preanalytical conditions for microrna profile analysis of clinical plasma samples
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9750036/
https://www.ncbi.nlm.nih.gov/pubmed/36516194
http://dx.doi.org/10.1371/journal.pone.0278927
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