Development of affinity columns for the removal of high-abundance proteins in cerebrospinal fluid.
Artikel i vetenskaplig tidskrift, 2009

Various approaches for removal of high-abundance components in body fluids are currently available. While most methods are constructed for plasma depletion, there is a need for body-fluid-specific strategies. The aim of the present study was to design an affinity matrix suitable for the depletion of high-abundance proteins in CSF (cerebrospinal fluid). Hence, molecules with specific affinity towards proteins present at high concentration in CSF were desired. Affibody molecules are specific binders of small size that have shown high stability under various conditions and are therefore good candidates for such a matrix. The protein composition in CSF resembles that in plasma. However, 20% of the proteins are brain-derived and are therefore present in higher proportions in CSF than in plasma, whereas larger plasma-derived proteins are less abundant in CSF. Therefore five high-abundance CSF proteins were chosen for the design of a CSF-specific depletion setup. Affibody molecules with specificity towards HSA (human serum albumin), IgG, transferrin and transthyretin were combined in an affinity column. In addition, polyclonal antibodies against cystatin C were coupled to chromatographic beads and packed in a separate column. Highly reproducible and efficient removal of the five target proteins was observed. The proportion of depleted proteins were estimated to be 99, 95, 74, 92 and 83% for HSA, IgG, transferrin, transthyretin and cystatin C respectively. SDS/PAGE analysis was used for monitoring and identifying proteins in native CSF, depleted CSF samples and the captured fractions. Moreover, shotgun proteomics was used for protein identification in native as well as depleted CSF and the achieved data were compared. Enhanced identification of lower-abundance components was observed in the depleted fraction, in terms of more detected peptides per protein.

Cerebrospinal Fluid Proteins

Chromatography

Substrate Specificity

isolation & purification

Affinity

methods

Humans

metabolism

methods

metabolism

Antibodies

Polyacrylamide Gel

Analytic Sample Preparation Methods

Spectrometry

Enzyme-Linked Immunosorbent Assay

Electrophoresis

Matrix-Assisted Laser Desorption-Ionization

Mass

Författare

Margareta Ramström

Aida Zuberovic

Caroline Grönwall

Jörg Hanrieder

Göteborgs universitet

Jonas Bergquist

Sophia Hober

Biotechnology and Applied Biochemistry

0885-4513 (ISSN) 1470-8744 (eISSN)

Vol. 52 Pt 2 159-66

Ämneskategorier

Biokemi och molekylärbiologi

Analytisk kemi

Medicinsk bioteknologi (med inriktning mot cellbiologi (inklusive stamcellsbiologi), molekylärbiologi, mikrobiologi, biokemi eller biofarmaci)

DOI

10.1042/BA20080015

PubMed

18412540

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Skapat

2017-10-10