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Nanobead-based single-molecule pulldown for single cells

Investigation of cell-to-cell variability holds critical physiological and clinical implications. Thus, numerous new techniques have been developed for studying cell-to-cell variability, and these single-cell techniques can also be used to investigate rare cells. Moreover, for studying protein-prote...

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Autores principales: Zhao, Qirui, Shen, Yusheng, Li, Xiaofen, Li, Yulin, Tian, Fang, Yu, Xiaojie, Liu, Zhengzhao, Tong, Rongbiao, Park, Hyokeun, Yobas, Levent, Huang, Pingbo
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Elsevier 2023
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10679481/
https://www.ncbi.nlm.nih.gov/pubmed/38027957
http://dx.doi.org/10.1016/j.heliyon.2023.e22306
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author Zhao, Qirui
Shen, Yusheng
Li, Xiaofen
Li, Yulin
Tian, Fang
Yu, Xiaojie
Liu, Zhengzhao
Tong, Rongbiao
Park, Hyokeun
Yobas, Levent
Huang, Pingbo
author_facet Zhao, Qirui
Shen, Yusheng
Li, Xiaofen
Li, Yulin
Tian, Fang
Yu, Xiaojie
Liu, Zhengzhao
Tong, Rongbiao
Park, Hyokeun
Yobas, Levent
Huang, Pingbo
author_sort Zhao, Qirui
collection PubMed
description Investigation of cell-to-cell variability holds critical physiological and clinical implications. Thus, numerous new techniques have been developed for studying cell-to-cell variability, and these single-cell techniques can also be used to investigate rare cells. Moreover, for studying protein-protein interactions (PPIs) in single cells, several techniques have been developed based on the principle of the single-molecule pulldown (SiMPull) assay. However, the applicability of these single-cell SiMPull (sc-SiMPull) techniques is limited because of their high technical barrier and special requirements for target cells and molecules. Here, we report a highly innovative nanobead-based approach for sc-SiMPull that is based on our recently developed microbead-based, improved version of SiMPull for cell populations. In our sc-SiMPull method, single cells are captured in microwells and lysed in situ, after which commercially available, pre-surface-functionalized magnetic nanobeads are placed in the microwells to specifically capture proteins of interest together with their binding partners from cell extracts; subsequently, the PPIs are examined under a microscope at the single-molecule level. Relative to previously published methods, nanobead-based sc-SiMPull is considerably faster, easier to use, more reproducible, and more versatile for distinct cell types and protein molecules, and yet provides similar sensitivity and signal-to-background ratio. These crucial features should enable universal application of our method to the study of PPIs in single cells.
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spelling pubmed-106794812023-11-14 Nanobead-based single-molecule pulldown for single cells Zhao, Qirui Shen, Yusheng Li, Xiaofen Li, Yulin Tian, Fang Yu, Xiaojie Liu, Zhengzhao Tong, Rongbiao Park, Hyokeun Yobas, Levent Huang, Pingbo Heliyon Research Article Investigation of cell-to-cell variability holds critical physiological and clinical implications. Thus, numerous new techniques have been developed for studying cell-to-cell variability, and these single-cell techniques can also be used to investigate rare cells. Moreover, for studying protein-protein interactions (PPIs) in single cells, several techniques have been developed based on the principle of the single-molecule pulldown (SiMPull) assay. However, the applicability of these single-cell SiMPull (sc-SiMPull) techniques is limited because of their high technical barrier and special requirements for target cells and molecules. Here, we report a highly innovative nanobead-based approach for sc-SiMPull that is based on our recently developed microbead-based, improved version of SiMPull for cell populations. In our sc-SiMPull method, single cells are captured in microwells and lysed in situ, after which commercially available, pre-surface-functionalized magnetic nanobeads are placed in the microwells to specifically capture proteins of interest together with their binding partners from cell extracts; subsequently, the PPIs are examined under a microscope at the single-molecule level. Relative to previously published methods, nanobead-based sc-SiMPull is considerably faster, easier to use, more reproducible, and more versatile for distinct cell types and protein molecules, and yet provides similar sensitivity and signal-to-background ratio. These crucial features should enable universal application of our method to the study of PPIs in single cells. Elsevier 2023-11-14 /pmc/articles/PMC10679481/ /pubmed/38027957 http://dx.doi.org/10.1016/j.heliyon.2023.e22306 Text en © 2023 The Authors https://creativecommons.org/licenses/by/4.0/This is an open access article under the CC BY license (http://creativecommons.org/licenses/by/4.0/).
spellingShingle Research Article
Zhao, Qirui
Shen, Yusheng
Li, Xiaofen
Li, Yulin
Tian, Fang
Yu, Xiaojie
Liu, Zhengzhao
Tong, Rongbiao
Park, Hyokeun
Yobas, Levent
Huang, Pingbo
Nanobead-based single-molecule pulldown for single cells
title Nanobead-based single-molecule pulldown for single cells
title_full Nanobead-based single-molecule pulldown for single cells
title_fullStr Nanobead-based single-molecule pulldown for single cells
title_full_unstemmed Nanobead-based single-molecule pulldown for single cells
title_short Nanobead-based single-molecule pulldown for single cells
title_sort nanobead-based single-molecule pulldown for single cells
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10679481/
https://www.ncbi.nlm.nih.gov/pubmed/38027957
http://dx.doi.org/10.1016/j.heliyon.2023.e22306
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