CIL:814, Homo sapiens, permanent cell line cell. In Cell Image Library

This culture of HeLa cells was grown, fixed and labeled directly on 35-mm plastic petri dishes (not on cover slips). To preserve the 3D structure of cells, cultures were fixed in formaldehyde vapors at room temperature over 20 min. Fixation was performed as follows: medium was completely aspirated,...

Full description

Bibliographic Details
Main Author: Gleiberman, Anatoli
Format: Dataset
Language:unknown
Published: UC San Diego Library Digital Collections 2021
Subjects:
apoptotic mitochondrial changes
ATP biosynthetic process
Homo sapiens
Triton
Orca
Online Access:https://dx.doi.org/10.6075/j0gx49sn
https://library.ucsd.edu/dc/object/bb4307234c
id ftdatacite:10.6075/j0gx49sn
record_format openpolar
spelling ftdatacite:10.6075/j0gx49sn 2023-05-15T17:53:53+02:00 CIL:814, Homo sapiens, permanent cell line cell. In Cell Image Library Gleiberman, Anatoli 2021 application/zip image/jpeg text/plain https://dx.doi.org/10.6075/j0gx49sn https://library.ucsd.edu/dc/object/bb4307234c unknown UC San Diego Library Digital Collections Creative Commons Zero v1.0 Universal https://creativecommons.org/publicdomain/zero/1.0/legalcode cc0-1.0 CC0 apoptotic mitochondrial changes ATP biosynthetic process Homo sapiens dataset Dataset 2021 ftdatacite https://doi.org/10.6075/j0gx49sn 2021-11-05T12:55:41Z This culture of HeLa cells was grown, fixed and labeled directly on 35-mm plastic petri dishes (not on cover slips). To preserve the 3D structure of cells, cultures were fixed in formaldehyde vapors at room temperature over 20 min. Fixation was performed as follows: medium was completely aspirated, a 50ul drop of 37% formaldehyde was placed on the lid of the dish and covered with the dish of cells, bottom up. After fixation dishes were carefully filled with 1ml of 50% glycerol in PBS and dishes were stored at -20 C until staining. Before staining, cells were incubated with blocking solution (5% fetal calf serum, PBS, 0.2% triton x-100, 25 min room temp.), then treated with primary antibody, which was mouse anti-Cytochrome C from BD Pharmigen (cat.# 556433) diluted 1:100 in blocking solution, 1h room temp. After standard washing (PBS 3-4 times, 5 min each), secondary antibody (donkey monovalent Fab-fragment anti-mouse IgG conjugated with Rhodamine Red-X from Jackson ImmunoResearch laboratories, concentration 2.5ug/ml) was applied. Images were captured on a Zeiss Axioplan-2. Objective - 63x oil immersion/NA 1.25. Magnifying lens (optovar) was 1.5. Digital camera – Hamamatsu ORCA-ER. Program – AxioVision 3.5.1. Illumination-mercury bulb HBP50. Filter set – standard for Rhodamine/Cy3/Alexa 564 – excitation 530-585 and emission LP 615. Mounting medium-VectaShield. Dataset Orca DataCite Metadata Store (German National Library of Science and Technology) Triton ENVELOPE(-55.615,-55.615,49.517,49.517)
institution Open Polar
collection DataCite Metadata Store (German National Library of Science and Technology)
op_collection_id ftdatacite
language unknown
topic apoptotic mitochondrial changes
ATP biosynthetic process
Homo sapiens
spellingShingle apoptotic mitochondrial changes
ATP biosynthetic process
Homo sapiens
Gleiberman, Anatoli
CIL:814, Homo sapiens, permanent cell line cell. In Cell Image Library
topic_facet apoptotic mitochondrial changes
ATP biosynthetic process
Homo sapiens
description This culture of HeLa cells was grown, fixed and labeled directly on 35-mm plastic petri dishes (not on cover slips). To preserve the 3D structure of cells, cultures were fixed in formaldehyde vapors at room temperature over 20 min. Fixation was performed as follows: medium was completely aspirated, a 50ul drop of 37% formaldehyde was placed on the lid of the dish and covered with the dish of cells, bottom up. After fixation dishes were carefully filled with 1ml of 50% glycerol in PBS and dishes were stored at -20 C until staining. Before staining, cells were incubated with blocking solution (5% fetal calf serum, PBS, 0.2% triton x-100, 25 min room temp.), then treated with primary antibody, which was mouse anti-Cytochrome C from BD Pharmigen (cat.# 556433) diluted 1:100 in blocking solution, 1h room temp. After standard washing (PBS 3-4 times, 5 min each), secondary antibody (donkey monovalent Fab-fragment anti-mouse IgG conjugated with Rhodamine Red-X from Jackson ImmunoResearch laboratories, concentration 2.5ug/ml) was applied. Images were captured on a Zeiss Axioplan-2. Objective - 63x oil immersion/NA 1.25. Magnifying lens (optovar) was 1.5. Digital camera – Hamamatsu ORCA-ER. Program – AxioVision 3.5.1. Illumination-mercury bulb HBP50. Filter set – standard for Rhodamine/Cy3/Alexa 564 – excitation 530-585 and emission LP 615. Mounting medium-VectaShield.
format Dataset
author Gleiberman, Anatoli
author_facet Gleiberman, Anatoli
author_sort Gleiberman, Anatoli
title CIL:814, Homo sapiens, permanent cell line cell. In Cell Image Library
title_short CIL:814, Homo sapiens, permanent cell line cell. In Cell Image Library
title_full CIL:814, Homo sapiens, permanent cell line cell. In Cell Image Library
title_fullStr CIL:814, Homo sapiens, permanent cell line cell. In Cell Image Library
title_full_unstemmed CIL:814, Homo sapiens, permanent cell line cell. In Cell Image Library
title_sort cil:814, homo sapiens, permanent cell line cell. in cell image library
publisher UC San Diego Library Digital Collections
publishDate 2021
url https://dx.doi.org/10.6075/j0gx49sn
https://library.ucsd.edu/dc/object/bb4307234c
long_lat ENVELOPE(-55.615,-55.615,49.517,49.517)
geographic Triton
geographic_facet Triton
genre Orca
genre_facet Orca
op_rights Creative Commons Zero v1.0 Universal
https://creativecommons.org/publicdomain/zero/1.0/legalcode
cc0-1.0
op_rightsnorm CC0
op_doi https://doi.org/10.6075/j0gx49sn
_version_ 1766161579539169280

Similar Items