Metabolic Syndrome Clinical Trial
Official title:
Mechanisms Underlying Metabolic Syndrome in Obesity
The purpose of this study is to better understand the link between obesity and diabetes or pre-diabetes.
Obesity is the most common and powerful force for creating insulin resistance and metabolic
syndrome, however, the molecular basis of this association is not well understood. In this
proposal, three independently funded researchers—Philip Kern, MD a clinical investigator,
and Charlotte Peterson, PhD and Robert McGehee, PhD, with significant experience in muscle
and adipocyte biology, respectively—will formalize a collaborative effort as a natural
extension of previous work and shared interests in the fields of obesity, insulin
resistance, and tissue lipid accumulation. Our overall hypothesis is that insulin resistance
in humans stems largely from ectopic accumulation of intramyocellular lipid (IMCL) during
the development of obesity. Further, we hypothesize that excess IMCL accumulation is
dependent on secretory proteins derived from a complex interplay between adipocytes and
macrophages in adipose tissue. To test these hypotheses, we will examine the interactions
among adipocytes, macrophages, and muscle cells isolated and cultured from subjects that are
obese with insulin resistance and impaired glucose tolerance (IGT), and from some with Type
2 Diabetes. This study population has elevated IMCL and is at high risk for obesity
complications, but avoids the pathophysiologic complications of glucotoxicity. These
subjects will be compared to obese subjects with normal glucose tolerance (NGT).
Aim 1 will explore mechanisms that contribute to IMCL and elucidate its role in the
development of IGT. Cultured muscle cells will be used to determine whether obese subjects
with IGT versus NGT demonstrate intrinsic differences in muscle gene expression and
metabolic activity under differing extracellular fatty acid concentrations. Lipid
accumulation and oxidation, and insulin-mediated glycogen synthesis and signaling will be
assessed.
Aim 2 will determine if the IMCL accumulation is dependent on adipose tissue secretory
proteins. We will use co-cultures of adipocytes, myoblasts, and adipose stromal vascular
cells to examine IMCL and the development of insulin resistance.
Aim 3 will determine whether the stromal fraction from IGT subjects promotes IMCL more
effectively than that from NGT subjects in co-cultures with muscle cells. We will compare
the stromal vascular fractions with regard to monocyte/macrophage accumulation and cytokine
expression.
Aim 4 will determine if improved glucose tolerance in response to a 10-week treatment with
pioglitazone results in decreased IMCL and identify cellular mechanisms involved. Co-culture
studies will also be used with muscle and stromal cells, before and after pioglitazone
treatment. These experiments will provide mechanistic insight into the link between obesity
and muscle function leading to metabolic syndrome.
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