IGF-IR signal transduction protein content and its activation by IGF-I in human placentas: relationship with gestational age and birth weight
Author
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Iñíguez Vila, Germán
Author
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Castro, Juan José
es_CL
Author
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García Mora, Mirna
es_CL
Author
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Kakarieka, Elena
es_CL
Author
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Johnson Pena, María Cecilia
es_CL
Author
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Cassorla Goluboff, Fernando
es_CL
Author
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Mericq, Verónica
es_CL
Admission date
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2015-01-06T12:52:54Z
Available date
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2015-01-06T12:52:54Z
Publication date
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2014
Cita de ítem
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PLOS One July 2014 | Volume 9 | Issue 7 | e102252
en_US
Identifier
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DOI: 10.1371/journal.pone.0102252
Identifier
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https://repositorio.uchile.cl/handle/2250/129542
General note
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Artículo de publicación ISI
en_US
Abstract
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Introduction: The human placenta expresses the IGF-I and IGF-IR proteins and their intracellular signal components (IRS-1,
AKT and mTOR). The aim of this study was to assess the IGF-IR content and activation of downstream signaling molecules in
placentas from newborns who were classified by gestational age and birth weight. We studied placentas from 25 term
appropriate (T-AGA), 26 term small (T-SGA), 22 preterm AGA (PT-AGA), and 20 preterm SGA (PT-SGA) newborns. The total
and phosphorylated IGF-IR, IRS-1, AKT, and mTOR contents were determined by Western Blot and normalized by actin or
with their respective total content. The effect of IGF-I was determined by stimulating placental explants with recombinant
IGF-I 10-8 mol/L for 15, 30, and 60 minutes.
Results: The IGF-IR content was higher in T-SGA compared to T-AGA placentas, and the IRS-1 content was higher in PTplacentas
compared with their respective T-placentas. The effect of IGF-I on the phosphorylated forms of IGF-IR was
increased in T-SGA (150%) and PT-SGA (300%) compared with their respective AGA placentas. In addition, AKT serine
phosphorylation was higher in PT-SGA compared to PT-AGA and T-SGA placentas (90% and 390% respectively).
Conclusion: The higher protein content and response to IGF-I of IGF-IR, IRS-1, and AKT observed in SGA placentas may
represent a compensatory mechanism in response to fetal growth restriction.
en_US
Patrocinador
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This work was supported by FONDECYT Grant 111 0240.