AKT and AMPK Activation after High-Fat and High-Glucose In Vitro Treatment of Prostate Epithelial Cells.

Ribeiro, D L; Góes, R M; Pinto-Fochi, M E; Taboga, S R; Abrahamsson, Per-Anders; Dizeyi, Nishtman

AKT and AMPK Activation after High-Fat and High-Glucose In Vitro Treatment of Prostate Epithelial Cells.

Mark

Ribeiro, D L ; Góes, R M ; Pinto-Fochi, M E ; Taboga, S R ; Abrahamsson, Per-Anders ^LU and Dizeyi, Nishtman ^LU (2014) In Hormone and Metabolic Research 46(7). p.471-476

Abstract: Considering the increasing consumption of saturated fat and glucose in diets worldwide and its possible association to carcinogenesis, this investigation analysed the proliferation profile of nonmalignant human prostate epithelial cells after exposure to elevated levels of fat and glucose. PNT1A cells were cultured with palmitate (100 or 200 μM) and/or glucose (450 mg/dl) for 24 or 48 h. Treated cells were evaluated for viability test and cell proliferation (MTS assay). AKT and AMPK phosphorylation status were analysed by Western blotting. After 24 h of high-fat alone or associated with high-glucose treatment, there was an increase in AMPK and AKT activation associated to unchanged MTS-cell proliferation. Following 48 h of high-fat but not... (More); Considering the increasing consumption of saturated fat and glucose in diets worldwide and its possible association to carcinogenesis, this investigation analysed the proliferation profile of nonmalignant human prostate epithelial cells after exposure to elevated levels of fat and glucose. PNT1A cells were cultured with palmitate (100 or 200 μM) and/or glucose (450 mg/dl) for 24 or 48 h. Treated cells were evaluated for viability test and cell proliferation (MTS assay). AKT and AMPK phosphorylation status were analysed by Western blotting. After 24 h of high-fat alone or associated with high-glucose treatment, there was an increase in AMPK and AKT activation associated to unchanged MTS-cell proliferation. Following 48 h of high-fat but not high-glucose alone, cells decreased AMPK activation and maintained elevated AKT levels. These data were associated to increased cell proliferation after further high-fat treatment. After longer high-fat exposure, MTS revealed that cells remained proliferating. High-glucose alone or associated to high-fat treatment was not able to increase cell proliferation and AKT activation. A high-fat medium containing 100 μM of palmitate stimulates proliferation in PNT1A cells by decreasing the activation of AMPK and increasing activation of AKT after longer exposure time. These findings improve the knowledge about the negative effect of high levels of this saturated fatty acid on proliferative disorders of prostate. (Less)

Please use this url to cite or link to this publication: https://lup.lub.lu.se/record/4455756

author

Ribeiro, D L ; Góes, R M ; Pinto-Fochi, M E ; Taboga, S R ; Abrahamsson, Per-Anders ^LU and Dizeyi, Nishtman ^LU

organization

Urological research, Malmö (research group)

publishing date

2014

type

Contribution to journal

publication status

published

subject

Urology and Nephrology

in

Hormone and Metabolic Research

volume

46

issue

7

pages

471 - 476

publisher

Georg Thieme Verlag

external identifiers

pmid:24799027
wos:000337172800003
scopus:84902532972
pmid:24799027

ISSN

1439-4286

DOI

10.1055/s-0034-1370991

language

English

LU publication?

yes

id

ecfadb78-d301-4405-b1b1-8ffa1e75a60d (old id 4455756)

alternative location

http://www.ncbi.nlm.nih.gov/pubmed/24799027?dopt=Abstract

date added to LUP

2016-04-01 11:16:37

date last changed

2022-02-18 01:28:35

@article{ecfadb78-d301-4405-b1b1-8ffa1e75a60d,
  abstract     = {{Considering the increasing consumption of saturated fat and glucose in diets worldwide and its possible association to carcinogenesis, this investigation analysed the proliferation profile of nonmalignant human prostate epithelial cells after exposure to elevated levels of fat and glucose. PNT1A cells were cultured with palmitate (100 or 200 μM) and/or glucose (450 mg/dl) for 24 or 48 h. Treated cells were evaluated for viability test and cell proliferation (MTS assay). AKT and AMPK phosphorylation status were analysed by Western blotting. After 24 h of high-fat alone or associated with high-glucose treatment, there was an increase in AMPK and AKT activation associated to unchanged MTS-cell proliferation. Following 48 h of high-fat but not high-glucose alone, cells decreased AMPK activation and maintained elevated AKT levels. These data were associated to increased cell proliferation after further high-fat treatment. After longer high-fat exposure, MTS revealed that cells remained proliferating. High-glucose alone or associated to high-fat treatment was not able to increase cell proliferation and AKT activation. A high-fat medium containing 100 μM of palmitate stimulates proliferation in PNT1A cells by decreasing the activation of AMPK and increasing activation of AKT after longer exposure time. These findings improve the knowledge about the negative effect of high levels of this saturated fatty acid on proliferative disorders of prostate.}},
  author       = {{Ribeiro, D L and Góes, R M and Pinto-Fochi, M E and Taboga, S R and Abrahamsson, Per-Anders and Dizeyi, Nishtman}},
  issn         = {{1439-4286}},
  language     = {{eng}},
  number       = {{7}},
  pages        = {{471--476}},
  publisher    = {{Georg Thieme Verlag}},
  series       = {{Hormone and Metabolic Research}},
  title        = {{AKT and AMPK Activation after High-Fat and High-Glucose In Vitro Treatment of Prostate Epithelial Cells.}},
  url          = {{http://dx.doi.org/10.1055/s-0034-1370991}},
  doi          = {{10.1055/s-0034-1370991}},
  volume       = {{46}},
  year         = {{2014}},
}

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AKT and AMPK Activation after High-Fat and High-Glucose In Vitro Treatment of Prostate Epithelial Cells.