Abstract

Flow cytometry is an important tool in quantifying and phenotyping the cells that define pathways relevant to diabetes. Previously limited to the analysis of circulating immune cells, advances in cell extraction from tissues has allowed flow cytometry to expand its capabilities to the study of developmental, metabolic and signaling programs in a wide-variety of cell types. The Cytometry & Cell Sorting Core (CCSC) has established itself as a vital and growing component of the Columbia University Diabetes Research Center (DRC), as it addressed the research needs of a growing number of DRC investigators who study immunological, developmental, and metabolic aspects of diabetes. Created in 2010 in partnership with the Columbia Center for Translational Immunology (CCTI) and the Department of Medicine (DOM) with a substantial University investment as well as NIH support, in the past 5 years CCSC has assisted 22 DRC users currently funded by 55 NIH grants, including 30 NIDDK grants. The data generated with the CCSC contributed to 63 publications and 17 new grants. The implementation of CCSC has been essential to support many aspects of diabetes research at Columbia. Since its establishment, the demand for CCSC services has steadily increased, from 60 hours per week with two analyzers to over 130 hours per week with three analyzers, and from 25 hours per week with one sorter to over 60 hours per week with two sorters. We expect usage to continue to grow as new recruits join the DRC, and established investigators take advantage of resources and technologies offered by the Core. Overall, CCSC will assist investigators with the following two aims:
Aim 1 ? To quantify and phenotypically characterize cell populations that contribute to the metabolic, immunologic and developmental programs of diabetes and its complications. CCSC leverages advanced technologies in fluorescent imaging at the single cell resolution to support the analysis of many different cell types in both human and animal tissues, as well as humanized mouse models of Type 1 diabetes.
Aim 2 ? To purify populations of cells of relevance to diabetes and its complications. Using fluorescence-activated cell sorting, CCSC supports DRC investigators to purify individual populations of cells for in vitro culture, in vivo implantation or molecular characterization including genetic and transcriptional profiling, protein purification and signaling studies, and for functional analysis including T cell activation, proliferation and migration studies. To achieve these aims, the CCSC has established standard operating procedures to: (i) Assure quality control and reproducibility; (ii) Prioritize investigator use; (iii) Monitor Core use; and (iv) Adapt to new technologies and to the needs of the Columbia Research Base.

Public Health Relevance

Flow cytometry is an important tool in quantifying and phenotyping the cells that define pathways relevant to diabetes. The implementation of the Cytometry and Cell Sorting Core has been essential to support many aspects of diabetes research that require quantification and phenotypic characterization of cell populations that contribute to the metabolic, immunologic and developmental programs of diabetes and its complications.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Diabetes and Digestive and Kidney Diseases (NIDDK)
Type
Center Core Grants (P30)
Project #
5P30DK063608-19
Application #
10104486
Study Section
Special Emphasis Panel (ZDK1)
Project Start
2020-02-01
Project End
2023-01-31
Budget Start
2021-02-01
Budget End
2022-01-31
Support Year
19
Fiscal Year
2021
Total Cost
Indirect Cost

  Institution

Name
Columbia University (N.Y.)
Department
Type
DUNS #
621889815
City
New York
State
NY
Country
United States
Zip Code
10032

  Publications

Sui, Lina; Danzl, Nichole; Campbell, Sean R et al. (2018) ?-Cell Replacement in Mice Using Human Type 1 Diabetes Nuclear Transfer Embryonic Stem Cells. Diabetes 67:26-35
Laferrère, Blandine; Pattou, François (2018) Weight-Independent Mechanisms of Glucose Control After Roux-en-Y Gastric Bypass. Front Endocrinol (Lausanne) 9:530
Shah, Ankit; Levesque, Kiarra; Pierini, Esmeralda et al. (2018) Effect of sitagliptin on glucose control in type 2 diabetes mellitus after Roux-en-Y gastric bypass surgery. Diabetes Obes Metab 20:1018-1023
Haeusler, Rebecca A; McGraw, Timothy E; Accili, Domenico (2018) Biochemical and cellular properties of insulin receptor signalling. Nat Rev Mol Cell Biol 19:31-44
Kraakman, Michael J; Liu, Qiongming; Postigo-Fernandez, Jorge et al. (2018) PPAR? deacetylation dissociates thiazolidinedione's metabolic benefits from its adverse effects. J Clin Invest 128:2600-2612
Kumar, Brahma V; Kratchmarov, Radomir; Miron, Michelle et al. (2018) Functional heterogeneity of human tissue-resident memory T cells based on dye efflux capacities. JCI Insight 3:
Ghorpade, Devram S; Ozcan, Lale; Zheng, Ze et al. (2018) Hepatocyte-secreted DPP4 in obesity promotes adipose inflammation and insulin resistance. Nature 555:673-677
Connors, Thomas J; Baird, J Scott; Yopes, Margot C et al. (2018) Developmental Regulation of Effector and Resident Memory T Cell Generation during Pediatric Viral Respiratory Tract Infection. J Immunol 201:432-439
Savage, Thomas M; Shonts, Brittany A; Obradovic, Aleksandar et al. (2018) Early expansion of donor-specific Tregs in tolerant kidney transplant recipients. JCI Insight 3:
Molusky, Matthew M; Hsieh, Joanne; Lee, Samuel X et al. (2018) Metformin and AMP Kinase Activation Increase Expression of the Sterol Transporters ABCG5/8 (ATP-Binding Cassette Transporter G5/G8) With Potential Antiatherogenic Consequences. Arterioscler Thromb Vasc Biol 38:1493-1503

Showing the most recent 10 out of 225 publications