Abstract

Elevated levels of glucose and/or lipids in Type 2 diabetes (T2DM) are thought to negatively affect islet function and survival (so-called `glucotoxicity', `lipotoxicity', or `gluco-lipotoxiciy'), leading to a further impairment of insulin secretion and worsening glycemic control. However, much of the evidence for glucotoxicity or lipotoxicity has come from studies of rodent islets or rodent models of T2DM (ob/ob, db/db, ZDF, high-fat diet, etc.). This is problematic because human islets have critical differences from rodent islets. Thus, our understanding of the mechanistic events in human islets exposed to excess glucose and lipid in vivo is quite limited. These fundamental gaps in our knowledge, which are partly the result of experimental limitations of studying human islets in vivo and partly from limitations in our knowledge of human islet biology, restrict our ability to develop interventions to preserve beta cell function. To address these limitations, we developed new pre-clinical, experimental approaches that allow mechanistic analysis of human islets exposed to excess glucose and/or lipid in vivo (human islets transplanted into immunodeficient mice). Based on our in vivo and in vitro data, we hypothesize that excess glucose and/or lipid in vivo (glucotoxicity or lipotoxicity) compromises the function and/or expression of these key islet-enriched transcription factors in human islets, leading to impaired insulin secretion and biosynthesis and the worsening islet function in T2DM. We propose three aims to test this hypothesis: 1) Define the degree, duration, and mechanism(s) by which hyperglycemia alters human islet function in vivo. 2) Determine whether excess lipid worsens the effects of hyperglycemia on human islet function in vivo. 3) Determine whether excess glucose and/or lipid impair human islet function in vivo by similar or distinct mechanisms. The proposed studies bring together new information and technologies related to islet-enriched transcription factors and human islet biology, as well as new experimental models that allow for human islets to be studied in vivo in ways that have not previously been possible. The proposed studies address a critical problem in T2DM, namely the molecular mechanisms of glucotoxicity and/or lipotoxicity, and should drive new efforts to design interventions to preserve or improve beta cell function.

Public Health Relevance

Type 2 diabetes is a major health challenge in the VA population. Elevated levels of glucose and/or lipid (fat) in type 2 diabetes lead to a further impairment of insulin release, and this creates a cycle that worsens diabetes control (sometimes called glucose or lipid toxicity). Much of our knowledge about glucose or lipid toxicity has come from studies of rodent cells or rodents with diabetes. This is problematic because human islets have critical differences from rodent islets. In this grant, we will use new information, technologies, and experimental approaches that allow studies of human islets in a similar situation to islets in people and that enable studis not previously possible. The proposed studies should improve our understanding of why type 2 diabetes develops and help efforts to design new therapies.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
Veterans Affairs (VA)
Type
Non-HHS Research Projects (I01)
Project #
5I01BX000666-07
Application #
9486831
Study Section
Endocriniology A (ENDA)
Project Start
2009-10-01
Project End
2019-09-30
Budget Start
2017-10-01
Budget End
2018-09-30
Support Year
7
Fiscal Year
2018
Total Cost
Indirect Cost

  Institution

Name
Veterans Health Administration
Department
Type
DUNS #
156385783
City
Nashville
State
TN
Country
United States
Zip Code
37212

  Publications

Brissova, Marcela; Haliyur, Rachana; Saunders, Diane et al. (2018) ? Cell Function and Gene Expression Are Compromised in Type 1 Diabetes. Cell Rep 22:2667-2676
Marre, Meghan L; McGinty, John W; Chow, I-Ting et al. (2018) Modifying Enzymes Are Elicited by ER Stress, Generating Epitopes That Are Selectively Recognized by CD4+ T Cells in Patients With Type 1 Diabetes. Diabetes 67:1356-1368
Dean, E Danielle; Li, Mingyu; Prasad, Nripesh et al. (2017) Interrupted Glucagon Signaling Reveals Hepatic ? Cell Axis and Role for L-Glutamine in ? Cell Proliferation. Cell Metab 25:1362-1373.e5
Bozadjieva, Nadejda; Blandino-Rosano, Manuel; Chase, Jennifer et al. (2017) Loss of mTORC1 signaling alters pancreatic ? cell mass and impairs glucagon secretion. J Clin Invest 127:4379-4393
Aamodt, Kristie I; Powers, Alvin C (2017) Signals in the pancreatic islet microenvironment influence ?-cell proliferation. Diabetes Obes Metab 19 Suppl 1:124-136
Arda, H Efsun; Li, Lingyu; Tsai, Jennifer et al. (2016) Age-Dependent Pancreatic Gene Regulation Reveals Mechanisms Governing Human ? Cell Function. Cell Metab 23:909-20
Delong, Thomas; Wiles, Timothy A; Baker, Rocky L et al. (2016) Pathogenic CD4 T cells in type 1 diabetes recognize epitopes formed by peptide fusion. Science 351:711-4
Ceddia, Ryan P; Lee, DaeKee; Maulis, Matthew F et al. (2016) The PGE2 EP3 Receptor Regulates Diet-Induced Adiposity in Male Mice. Endocrinology 157:220-32
Boortz, Kayla A; Syring, Kristen E; Dai, Chunhua et al. (2016) G6PC2 Modulates Fasting Blood Glucose In Male Mice in Response to Stress. Endocrinology 157:3002-8
Dai, Chunhua; Kayton, Nora S; Shostak, Alena et al. (2016) Stress-impaired transcription factor expression and insulin secretion in transplanted human islets. J Clin Invest 126:1857-70

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