A novel quantitative assay for analysis of GLUT4 translocation using high content screening

SaiSantosh Babu Komakula; Ashok Kumar Tiwari; Shashi Singh

doi:10.1016/j.biopha.2020.111032

A novel quantitative assay for analysis of GLUT4 translocation using high content screening

Biomed Pharmacother. 2021 Jan:133:111032. doi: 10.1016/j.biopha.2020.111032. Epub 2020 Dec 1.

Authors

SaiSantosh Babu Komakula¹, Ashok Kumar Tiwari², Shashi Singh³

Affiliations

¹ CSIR-Centre for Cellular and Molecular Biology, Hyderabad, India; Department of Experimental Biology, Wrocław University of Environmental and Life Sciences, Wroclaw, Poland.
² CSIR- Indian Institute of Chemical Technology, Hyderabad, India.
³ CSIR-Centre for Cellular and Molecular Biology, Hyderabad, India. Electronic address: shashis@ccmb.res.in.

PMID: 33378945
DOI: 10.1016/j.biopha.2020.111032

Abstract

Insulin resistance is associated with obesity and can lead to several metabolic disorders including type II diabetes, nonalcoholic fatty liver disease and cardiovascular problems. Search for the small molecules which can either induce or mimic the insulin action are of great interest and can be utilized to manage insulin resistance. There are several dietary phytochemicals which can potentially have insulinomimetic action. Nevertheless, high throughput screening methods to test efficiency of small molecules to act as an insulinomimetic are not fully established. In this paper we have performed chemical screen analysis based on GLUT4 translocation using a cell line CHO-HIRC-myc-GLUT4 eGFP that expresses GLUT4-GFP in association with human Insulin receptor. We have established a high content screening-based method which can track and quantify the GLUT4 translocation from perinuclear area to the cell membrane. The assay involves measuring fluorescence intensity in a defined perinuclear area and a defined area along the cell membrane; and the results are expressed as the ratio of fluorescence intensity in the perinuclear to membrane area. The assay could collect real time data of GLUT4 translocation from thousand of cells/ sample and from many such samples in one experiment. We validated the assay using Insulin, insulin mimics/sensitizers and insulin inhibitors. The agonist or antagonists were analyzed for their ability to enhance or block the GLUT4 translocation independent of insulin. The outcome of the assay was correlated by performing glucose uptake assay using differentiated 3T3L1 cells. Using this platform we further identified several plant extracts which had the insulin mimetic action. We confirmed that these plant extracts were non-toxic to the beta cells using RIN mf5cells and 3T3L1 cells. We have identified plant extracts with the potential insulinomimetic action using novel high-content screening approach; these can be further tested for their efficiency in-vivo in pre-clinical trials.

Keywords: Cell based assay; GLUT4-GFP; Insulin sensitizers; Insulinomimetics; Membrane translocation; Phytochemicals; Screening.

Publication types

Comparative Study

MeSH terms

3T3 Cells
Adipocytes / drug effects
Adipocytes / metabolism*
Animals
Biological Assay*
CHO Cells
Cricetulus
Glucose Transporter Type 4 / genetics
Glucose Transporter Type 4 / metabolism*
Hep G2 Cells
Hepatocytes / drug effects
Hepatocytes / metabolism*
High-Throughput Screening Assays*
Humans
Hypoglycemic Agents / pharmacology
Insulin / pharmacology
Insulin Resistance
Mice
Protein Transport / drug effects
Reproducibility of Results
Time Factors

Substances

Glucose Transporter Type 4
Hypoglycemic Agents
Insulin
SLC2A4 protein, human
Slc2a4 protein, mouse