Biophysical characterization data on Aβ soluble oligomers produced through a method enabling prolonged oligomer stability and biological buffer conditions

The data here consists of time-dependent experimental parameters from chemical and biophysical methods used to characterize Aβ monomeric reactants as well as soluble oligomer and amyloid fibril products from a slow (3–4 week) assembly reaction under biologically-relevant solvent conditions. The data...

Descripción completa

Detalles Bibliográficos
Autores principales: Crisostomo, Amanda C., Dang, Loan, Digambaranath, Jyothi L., Klaver, Andrea C., Loeffler, David A., Payne, Jeremiah J., Smith, Lynnae M., Yokom, Adam L., Finke, John M.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Elsevier 2015
Materias:
Data Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4560727/
https://www.ncbi.nlm.nih.gov/pubmed/26401521
http://dx.doi.org/10.1016/j.dib.2015.07.034
_version_ 1782388949022408704
author Crisostomo, Amanda C.
Dang, Loan
Digambaranath, Jyothi L.
Klaver, Andrea C.
Loeffler, David A.
Payne, Jeremiah J.
Smith, Lynnae M.
Yokom, Adam L.
Finke, John M.
author_facet Crisostomo, Amanda C.
Dang, Loan
Digambaranath, Jyothi L.
Klaver, Andrea C.
Loeffler, David A.
Payne, Jeremiah J.
Smith, Lynnae M.
Yokom, Adam L.
Finke, John M.
author_sort Crisostomo, Amanda C.
collection PubMed
description The data here consists of time-dependent experimental parameters from chemical and biophysical methods used to characterize Aβ monomeric reactants as well as soluble oligomer and amyloid fibril products from a slow (3–4 week) assembly reaction under biologically-relevant solvent conditions. The data of this reaction are both of a qualitative and quantitative nature, including gel images from chemical cross-linking and Western blots, fractional solubility, thioflavin T binding, size exclusion chromatograms, transmission electron microscopy images, circular dichroism spectra, and fluorescence resonance energy transfer efficiencies of donor–acceptor pair labels in the Aβ chain. This data enables future efforts to produce the initial monomer and eventual soluble oligomer and amyloid fibril states by providing reference benchmarks of these states pertaining to physical properties (solubility), ligand-binding (thioflavin T binding), mesoscopic structure (electron microscopy, size exclusion chromatography, cross-linking products, SDS and native gels) and molecular structure (circular dichroism, FRET donor-acceptor distance). Aβ1-40 soluble oligomers are produced that are suitable for biophysical studies requiring sufficient transient stability to exist in their “native” conformation in biological phosphate-saline buffers for extended periods of time. The production involves an initial preparation of highly monomeric Aβ in a phosphate saline buffer that transitions to fibrils and oligomers through time incubation alone, without added detergents or non-aqueous chemicals. This criteria ensures that the only difference between initial monomeric Aβ reactant and subsequent Aβ oligomer products is their degree of peptide assembly. A number of chemical and biophysical methods were used to characterize the monomeric reactants and soluble oligomer and amyloid fibril products, including chemical cross-linking, Western blots, fraction solubility, thioflvain T binding, size exclusion chromatography, transmission electron micrscopy, circular dichroism spectroscopy, and fluorescence resonance energy transfer.
format Online
Article
Text
id pubmed-4560727
institution National Center for Biotechnology Information
language English
publishDate 2015
publisher Elsevier
record_format MEDLINE/PubMed
spelling pubmed-45607272015-09-23 Biophysical characterization data on Aβ soluble oligomers produced through a method enabling prolonged oligomer stability and biological buffer conditions Crisostomo, Amanda C. Dang, Loan Digambaranath, Jyothi L. Klaver, Andrea C. Loeffler, David A. Payne, Jeremiah J. Smith, Lynnae M. Yokom, Adam L. Finke, John M. Data Brief Data Article The data here consists of time-dependent experimental parameters from chemical and biophysical methods used to characterize Aβ monomeric reactants as well as soluble oligomer and amyloid fibril products from a slow (3–4 week) assembly reaction under biologically-relevant solvent conditions. The data of this reaction are both of a qualitative and quantitative nature, including gel images from chemical cross-linking and Western blots, fractional solubility, thioflavin T binding, size exclusion chromatograms, transmission electron microscopy images, circular dichroism spectra, and fluorescence resonance energy transfer efficiencies of donor–acceptor pair labels in the Aβ chain. This data enables future efforts to produce the initial monomer and eventual soluble oligomer and amyloid fibril states by providing reference benchmarks of these states pertaining to physical properties (solubility), ligand-binding (thioflavin T binding), mesoscopic structure (electron microscopy, size exclusion chromatography, cross-linking products, SDS and native gels) and molecular structure (circular dichroism, FRET donor-acceptor distance). Aβ1-40 soluble oligomers are produced that are suitable for biophysical studies requiring sufficient transient stability to exist in their “native” conformation in biological phosphate-saline buffers for extended periods of time. The production involves an initial preparation of highly monomeric Aβ in a phosphate saline buffer that transitions to fibrils and oligomers through time incubation alone, without added detergents or non-aqueous chemicals. This criteria ensures that the only difference between initial monomeric Aβ reactant and subsequent Aβ oligomer products is their degree of peptide assembly. A number of chemical and biophysical methods were used to characterize the monomeric reactants and soluble oligomer and amyloid fibril products, including chemical cross-linking, Western blots, fraction solubility, thioflvain T binding, size exclusion chromatography, transmission electron micrscopy, circular dichroism spectroscopy, and fluorescence resonance energy transfer. Elsevier 2015-08-06 /pmc/articles/PMC4560727/ /pubmed/26401521 http://dx.doi.org/10.1016/j.dib.2015.07.034 Text en © 2015 The Authors http://creativecommons.org/licenses/by/4.0/ This is an open access article under the CC BY license (http://creativecommons.org/licenses/by/4.0/).
spellingShingle Data Article
Crisostomo, Amanda C.
Dang, Loan
Digambaranath, Jyothi L.
Klaver, Andrea C.
Loeffler, David A.
Payne, Jeremiah J.
Smith, Lynnae M.
Yokom, Adam L.
Finke, John M.
Biophysical characterization data on Aβ soluble oligomers produced through a method enabling prolonged oligomer stability and biological buffer conditions
title Biophysical characterization data on Aβ soluble oligomers produced through a method enabling prolonged oligomer stability and biological buffer conditions
title_full Biophysical characterization data on Aβ soluble oligomers produced through a method enabling prolonged oligomer stability and biological buffer conditions
title_fullStr Biophysical characterization data on Aβ soluble oligomers produced through a method enabling prolonged oligomer stability and biological buffer conditions
title_full_unstemmed Biophysical characterization data on Aβ soluble oligomers produced through a method enabling prolonged oligomer stability and biological buffer conditions
title_short Biophysical characterization data on Aβ soluble oligomers produced through a method enabling prolonged oligomer stability and biological buffer conditions
title_sort biophysical characterization data on aβ soluble oligomers produced through a method enabling prolonged oligomer stability and biological buffer conditions
topic Data Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4560727/
https://www.ncbi.nlm.nih.gov/pubmed/26401521
http://dx.doi.org/10.1016/j.dib.2015.07.034
work_keys_str_mv AT crisostomoamandac biophysicalcharacterizationdataonabsolubleoligomersproducedthroughamethodenablingprolongedoligomerstabilityandbiologicalbufferconditions
AT dangloan biophysicalcharacterizationdataonabsolubleoligomersproducedthroughamethodenablingprolongedoligomerstabilityandbiologicalbufferconditions
AT digambaranathjyothil biophysicalcharacterizationdataonabsolubleoligomersproducedthroughamethodenablingprolongedoligomerstabilityandbiologicalbufferconditions
AT klaverandreac biophysicalcharacterizationdataonabsolubleoligomersproducedthroughamethodenablingprolongedoligomerstabilityandbiologicalbufferconditions
AT loefflerdavida biophysicalcharacterizationdataonabsolubleoligomersproducedthroughamethodenablingprolongedoligomerstabilityandbiologicalbufferconditions
AT paynejeremiahj biophysicalcharacterizationdataonabsolubleoligomersproducedthroughamethodenablingprolongedoligomerstabilityandbiologicalbufferconditions
AT smithlynnaem biophysicalcharacterizationdataonabsolubleoligomersproducedthroughamethodenablingprolongedoligomerstabilityandbiologicalbufferconditions
AT yokomadaml biophysicalcharacterizationdataonabsolubleoligomersproducedthroughamethodenablingprolongedoligomerstabilityandbiologicalbufferconditions
AT finkejohnm biophysicalcharacterizationdataonabsolubleoligomersproducedthroughamethodenablingprolongedoligomerstabilityandbiologicalbufferconditions

Ejemplares similares