2014
DOI: 10.3389/fncel.2014.00004
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Cryoloading: introducing large molecules into live synaptosomes

Abstract: Neurons communicate with their target cells primarily by the release of chemical transmitters from presynaptic nerve terminals. The study of CNS presynaptic nerve terminals, isolated as synaptosomes (SSMs) has, however, been hampered by the typical small size of these structures that precludes the introduction of non-membrane permeable test substances such as peptides and drugs. We have developed a method to introduce large alien compounds of at least 150 kDa into functional synaptosomes. Purified synaptosomes… Show more

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Cited by 9 publications
(27 citation statements)
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“…This hypothesis was tested in the chick SSMs using our novel “cryoloading” method (Nath et al, 2014) that permits the introduction of large (up to at least 150 kD) membrane-impermeable alien compounds into functional SSMs. Briefly, fresh SSMs were frozen in a buffer containing the test compound, a 3 kD dextran-FITC loading marker and a cryoprotectant.…”
Section: Resultsmentioning
confidence: 99%
“…This hypothesis was tested in the chick SSMs using our novel “cryoloading” method (Nath et al, 2014) that permits the introduction of large (up to at least 150 kD) membrane-impermeable alien compounds into functional SSMs. Briefly, fresh SSMs were frozen in a buffer containing the test compound, a 3 kD dextran-FITC loading marker and a cryoprotectant.…”
Section: Resultsmentioning
confidence: 99%
“…At 28 days after PSNL, one set of rats (n = 4 or 6 for each group) was sacrificed by an overdose of chloral hydrate (80 mg/kg). Immunohistochemical staining for GluR1, GluR2, NR1, NR2A, NR2B, and p-ERK1/2 was performed as described in previous studies [ 15 , 29 - 31 ] with a slight modification. Briefly, brains were fixed for 4 h in 4% paraformaldehyde after perfusion and cryoprotection by immersion in 20% sucrose in phosphate buffer (pH = 7.4) overnight.…”
Section: Methodsmentioning
confidence: 99%
“…The first concern was that a significant fraction of the synaptosomes may have resealed after the osmotic shock step, occluding antibody access to the luminal face of the AZ. This concern was solved by freeze-thaw-loading of the antibodies into the resealed synaptosomes using a protocol that we term cryoloading as described recently in detail (Nath et al, 2014). To improve labeling efficiency, we used a cocktail of L4569 and L4570, termed here L45, that is in effect a more heterogeneous polyclonal antibody than either alone.…”
Section: Resultsmentioning
confidence: 99%
“…To improve our signal to noise ratio, we made two key improvements to the gold labeling method. First, we used cryoloading (Nath et al, 2014) to freeze-load the synaptosome ghosts with the antibodies. Second, we replaced the conventional colloidal gold secondary antibody with Fab fragments that are covalently tagged with nanogold particles.…”
Section: Discussionmentioning
confidence: 99%
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