4.6 Article

Stoichiometric Analysis of Shifting in Subcellular Compartmentalization of HSP70 within Ischemic Penumbra

期刊

MOLECULES
卷 26, 期 12, 页码 -

出版社

MDPI
DOI: 10.3390/molecules26123578

关键词

mitochondria; autophagy-related vacuoles; chaperones; area penumbra; brain ischemia; transmission electron microscopy; quantitative morphometry; stoichiometric ultrastructural molecule detection

资金

  1. Ministero della Salute
  2. University of Pisa (Fondi di Ateneo)

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The heat shock protein (HSP) 70 plays a crucial role in neuronal survival in ischemic conditions, with high density found in cytosolic vacuoles and mitochondria in control conditions. However, a loss of such specific polarization is documented within the peri-infarct region, leading to depletion of HSP70 from these organelles. This may significantly impact the physiological functions of HSP70 in promoting neuronal survival.
The heat shock protein (HSP) 70 is considered the main hallmark in preclinical studies to stain the peri-infarct region defined area penumbra in preclinical models of brain ischemia. This protein is also considered as a potential disease modifier, which may improve the outcome of ischemic damage. In fact, the molecule HSP70 acts as a chaperonine being able to impact at several level the homeostasis of neurons. Despite being used routinely to stain area penumbra in light microscopy, the subcellular placement of this protein within area penumbra neurons, to our knowledge, remains undefined. This is key mostly when considering studies aimed at deciphering the functional role of this protein as a determinant of neuronal survival. The general subcellular placement of HSP70 was grossly reported in studies using confocal microscopy, although no direct visualization of this molecule at electron microscopy was carried out. The present study aims to provide a direct evidence of HSP70 within various subcellular compartments. In detail, by using ultrastructural morphometry to quantify HSP70 stoichiometrically detected by immuno-gold within specific organelles we could compare the compartmentalization of the molecule within area penumbra compared with control brain areas. The study indicates that two cell compartments in control conditions own a high density of HSP70, cytosolic vacuoles and mitochondria. In these organelles, HSP70 is present in amount exceeding several-fold the presence in the cytosol. Remarkably, within area penumbra a loss of such a specific polarization is documented. This leads to the depletion of HSP70 from mitochondria and mostly cell vacuoles. Such an effect is expected to lead to significant variations in the ability of HSP70 to exert its physiological roles. The present findings, beyond defining the neuronal compartmentalization of HSP70 within area penumbra may lead to a better comprehension of its beneficial/detrimental role in promoting neuronal survival.

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