A new approach to analysis of intracellular proteins and subcellular localization using cellprofiler and imageJ in combination

Akito Hattori; Etsuro Ohta; Makiko Nagai; Kazuya Iwabuchi; Hideyuki Okano

doi:10.1016/j.ymeth.2021.04.019

A new approach to analysis of intracellular proteins and subcellular localization using cellprofiler and imageJ in combination

Methods. 2022 Jul:203:233-241. doi: 10.1016/j.ymeth.2021.04.019. Epub 2021 Apr 26.

Authors

Akito Hattori¹, Etsuro Ohta², Makiko Nagai³, Kazuya Iwabuchi¹, Hideyuki Okano⁴

Affiliations

¹ Program in Cellular Immunology, Graduate School of Medical Science, Kitasato University, Kanagawa, Japan.
² R & D Center for Cell Design, Institute for Regenerative Medicine and Cell Design, Kitasato University School of Allied Health Sciences,Kanagawa, Japan; Department of ImmunologyⅡ, Kitasato University of Allied Health Science, Kanagawa, Japan; Division of Clinical Immunology, Graduate School of Medical Science, Kitasato University, Kanagawa, Japan; Department of Physiology, Keio University School of Medicine, Tokyo, Japan. Electronic address: eohta@kitasato-u.ac.jp.
³ Department of Neurology, Kitasato University School of Medicine, Kanagawa, Japan.
⁴ Department of Physiology, Keio University School of Medicine, Tokyo, Japan. Electronic address: hidokano@a2.keio.jp.

PMID: 33915291
DOI: 10.1016/j.ymeth.2021.04.019

Abstract

Analytical pipeline, which is used for various analysis application, of CellProfiler, an open-source software for cell imaging analysis, is very important. In the present study, to examine whether intracellular proteins can be discriminated using a combination of CellProfiler and ImageJ, we analyzed neuroblastoma and monocytic cell lines, and disease-specific induced pluripotent stem cell (iPSC)-derived neurons. This revealed that scattered puncta of Rab7 and transferrin in neuroblastoma lines were clearly detectable by created analytical pipelines in CellProfiler. We then constructed pipelines for measuring the distance from the center of the nucleus to allow investigation of the intracellular localization of Rab7 or transferrin. Using CellProfiler and ImageJ in combination, we confirmed that our pipelines were applicable both quantitatively and objectively to analysis of membrane trafficking of proteins such as Rab proteins and transferrin. In addition, when applied to quantitative measurement of phagocytosis, our pipelines clearly detected monocytic cell lines that had engulfed bioparticles. Finally, we developed new pipelines for analysis of disease phenotype using iPSCs from a patient with familial Parkinson's disease (PD), harboring the I2020T LRRK2 mutation (PARK8). These were able to successfully detect Rab5 puncta and Rab7 puncta in PARK8 patient iPSC-derived neurons. Interestingly, in long-term culture, we found that the numbers of Rab7 puncta in a single PARK8 patient iPSC-derived neurons were lower than that of control iPSC-derived neurons. On the other hands, at 14 days in vitro, the numbers of Rab5 puncta in PARK8 patient iPSC-derived neurons were lower than those of isogenic iPSC-derived neurons, but not Rab7 puncta. Furthermore, Rab5 puncta of PARK8 patient iPSC-derived neurons exhibited distinct localization pattern relative to isogenic iPSC-derived neurons. These present results suggest that this new analytical tool can be used as a supporting method for quantification of intracellular protein.

Keywords: Human induced pluripotent stem cell; Intracellular localization; Membrane-trafficking; Open-source image analysis software; Parkinson disease; Phagocytosis.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Cell Line
Humans
Induced Pluripotent Stem Cells*
Neuroblastoma* / metabolism
Neurons / metabolism
Transferrins / metabolism

Substances

Transferrins