A Novel Procedure for Pre-embedding Double Immunogold-Silver Labeling at the Ultrastructural Level

A Novel Procedure for Pre-embedding Double Immunogold-Silver Labeling at the Ultrastructural Level

Pre-embedding double immunogold–silver labeling using two ultrasmall gold conjugates has not been attempted previously because a means of distinguishing labels by conjugates of identical sizes was lacking. This study investigated the feasibility of creating a particle size segregation between two ul...

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Bibliographic Details
Published in:The journal of histochemistry and cytochemistry Vol. 49; no. 3; pp. 279 - 283
Main Authors: Yi, Hong, Leunissen, Jan L.M, Shi, Ge-Ming, Gutekunst, Claire-Anne, Hersch, Steven M
Format: Journal Article
Language:English
Published: Los Angeles, CA Histochemical Soc 01-03-2001
SAGE Publications
Subjects:
Animals
Antibodies
Brain - metabolism
Brain - ultrastructure
Glial Fibrillary Acidic Protein - immunology
Glial Fibrillary Acidic Protein - metabolism
Immunohistochemistry - methods
Mice
Mice, Inbred C57BL
Microscopy, Electron
Organelles - metabolism
Presynaptic Terminals - metabolism
Rabbits
Synaptophysin - immunology
Synaptophysin - metabolism
immunogold
electron microscopy
double labeling
pre-embedding labeling
silver enhancement
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Summary:Pre-embedding double immunogold–silver labeling using two ultrasmall gold conjugates has not been attempted previously because a means of distinguishing labels by conjugates of identical sizes was lacking. This study investigated the feasibility of creating a particle size segregation between two ultrasmall gold conjugates through sequential immunogold incubations and silver enhancements. Two primary antibodies, mouse anti-synaptophysin and rabbit anti-glial fibrillary acidic protein (GFAP), were used in the model system. Differentiation of the double labeling was achieved by incubating with one ultrasmall gold conjugate, followed by silver enhancement, and then incubating with the second ultrasmall gold conjugate, followed by additional silver enhancement. This resulted in two groups of silver-enhanced particles: smaller particles enhanced once and larger particles enhanced twice. Electron microscopic examination revealed two readily distinguished populations of gold–silver particles within the appropriate structures, with very little size overlap. The quality of the ultrastructure permitted identification of most subcellular organelles. This procedure provides for the first time a pre-embedding immunogold–silver labeling protocol that allows the precise subcellular co-localization of multiple antigens.
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ISSN:0022-1554
1551-5044
DOI:10.1177/002215540104900301