Scanning electron microscopy in liver biopsy interpretation in children: a mini atlas

Scanning electron microscopy in liver biopsy interpretation in children: a mini atlas

We have extensively studied the ultrastructural picture of the liver by scanning electron microscopy (SEM) but these studies were not used, up to now, in clinical practice because they were considered to be mainly a means of research in the 3D structure of liver specimens. Our new technique allows u...

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Main Authors: Cristina Mocci, Terenzio Congiu, Daniela Fanni, Clara Gerosa, Mina Komuta, Peter Van Eyken, Gavino Faa, Alessandro Riva
Format: Article
Language:English
Published: Hygeia Press di Corridori Marinella 2014-06-01
Series:Journal of Pediatric and Neonatal Individualized Medicine
Subjects:
sem
osmic maceration
liver biopsy
mitochondria
bile canaliculi
nucleus
Online Access:https://www.jpnim.com/index.php/jpnim/article/view/154
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spelling doaj-b2ccef29fb29423b9e82222eef3c42702020-11-25T03:31:18ZengHygeia Press di Corridori MarinellaJournal of Pediatric and Neonatal Individualized Medicine2281-06922014-06-0132e030206e03020610.7363/030206122Scanning electron microscopy in liver biopsy interpretation in children: a mini atlasCristina Mocci0Terenzio Congiu1Daniela Fanni2Clara Gerosa3Mina Komuta4Peter Van Eyken5Gavino Faa6Alessandro Riva7Department of Surgical Sciences, Division of Pathology, University of CagliariDepartment of Morphology, University of VareseDepartment of Surgical Sciences, Division of Pathology, University of CagliariDepartment of Surgical Sciences, Division of Pathology, University of CagliariDepartment of Pathology, University of LeuvenDepartment of Pathology, Ziekenhius Oost Limburg (ZOL), GenkDepartment of Surgical Sciences, Division of Pathology, University of CagliariDepartment of Pathology, Ziekenhius Oost Limburg (ZOL), GenkWe have extensively studied the ultrastructural picture of the liver by scanning electron microscopy (SEM) but these studies were not used, up to now, in clinical practice because they were considered to be mainly a means of research in the 3D structure of liver specimens. Our new technique allows us to introduce ourselves to the 3D structure of intracellular organelles, making it possible to study them in normal and pathologic conditions. We used a very small part of the liver biopsies from 5 children aged 3 to 8 years old, who underwent a liver biopsy for diagnostic purposes. The specimens were fixed and processed according to our modification of the OsO4 maceration method of Tanaka and Mitsushima. Liver biopsies fixed for 20’ in a mixture of glutaraldehyde and paraformaldehyde, postfixed in 1% OsO4 for 2 h, cut with a tissue sectioner and then macerated in 0.1% OsO4 for 60 h at room temperature. Specimens were dehydrated in graded acetone, critical point dried and coated with gold palladium. To selectively remove cell components, some specimens were subjected to ultrasound treatment (25 Hz for 1’) prior to dehydration. To demonstrate the hepatic stroma, some aldehyde-fixed specimens were submitted to maceration with NaOH 1N according to Ohtani method. With this method, all cells were removed, allowing the visualization of collagen fibers. Observation was carried out by an Hitachi S4000 Field Emission SEM (Hitachi High-Technologies Co., Tokyo, Japan) operated at 20 kV. We are showing the results of our new technique applied to the liver tissue. These data open, in our opinion, a new field in the research of nuclear pathology, with possible intriguing data on pathological nuclear pore changes in the setting of different liver diseases.https://www.jpnim.com/index.php/jpnim/article/view/154semosmic macerationliver biopsymitochondriabile canaliculinucleus
collection DOAJ
language English
format Article
sources DOAJ
author Cristina Mocci
Terenzio Congiu
Daniela Fanni
Clara Gerosa
Mina Komuta
Peter Van Eyken
Gavino Faa
Alessandro Riva
spellingShingle Cristina Mocci
Terenzio Congiu
Daniela Fanni
Clara Gerosa
Mina Komuta
Peter Van Eyken
Gavino Faa
Alessandro Riva
Scanning electron microscopy in liver biopsy interpretation in children: a mini atlas
Journal of Pediatric and Neonatal Individualized Medicine
sem
osmic maceration
liver biopsy
mitochondria
bile canaliculi
nucleus
author_facet Cristina Mocci
Terenzio Congiu
Daniela Fanni
Clara Gerosa
Mina Komuta
Peter Van Eyken
Gavino Faa
Alessandro Riva
author_sort Cristina Mocci
title Scanning electron microscopy in liver biopsy interpretation in children: a mini atlas
title_short Scanning electron microscopy in liver biopsy interpretation in children: a mini atlas
title_full Scanning electron microscopy in liver biopsy interpretation in children: a mini atlas
title_fullStr Scanning electron microscopy in liver biopsy interpretation in children: a mini atlas
title_full_unstemmed Scanning electron microscopy in liver biopsy interpretation in children: a mini atlas
title_sort scanning electron microscopy in liver biopsy interpretation in children: a mini atlas
publisher Hygeia Press di Corridori Marinella
series Journal of Pediatric and Neonatal Individualized Medicine
issn 2281-0692
publishDate 2014-06-01
description We have extensively studied the ultrastructural picture of the liver by scanning electron microscopy (SEM) but these studies were not used, up to now, in clinical practice because they were considered to be mainly a means of research in the 3D structure of liver specimens. Our new technique allows us to introduce ourselves to the 3D structure of intracellular organelles, making it possible to study them in normal and pathologic conditions. We used a very small part of the liver biopsies from 5 children aged 3 to 8 years old, who underwent a liver biopsy for diagnostic purposes. The specimens were fixed and processed according to our modification of the OsO4 maceration method of Tanaka and Mitsushima. Liver biopsies fixed for 20’ in a mixture of glutaraldehyde and paraformaldehyde, postfixed in 1% OsO4 for 2 h, cut with a tissue sectioner and then macerated in 0.1% OsO4 for 60 h at room temperature. Specimens were dehydrated in graded acetone, critical point dried and coated with gold palladium. To selectively remove cell components, some specimens were subjected to ultrasound treatment (25 Hz for 1’) prior to dehydration. To demonstrate the hepatic stroma, some aldehyde-fixed specimens were submitted to maceration with NaOH 1N according to Ohtani method. With this method, all cells were removed, allowing the visualization of collagen fibers. Observation was carried out by an Hitachi S4000 Field Emission SEM (Hitachi High-Technologies Co., Tokyo, Japan) operated at 20 kV. We are showing the results of our new technique applied to the liver tissue. These data open, in our opinion, a new field in the research of nuclear pathology, with possible intriguing data on pathological nuclear pore changes in the setting of different liver diseases.
topic sem
osmic maceration
liver biopsy
mitochondria
bile canaliculi
nucleus
url https://www.jpnim.com/index.php/jpnim/article/view/154
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