Laboratory methods to improve SELDI peak detection and quantitation

Rollin, Dominique; Whistler, Toni; Vernon, Suzanne D

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CDC STACKS serves as an archival repository of CDC-published products including scientific findings, journal articles, guidelines, recommendations, or other public health information authored or co-authored by CDC or funded partners. As a repository, CDC STACKS retains documents in their original published format to ensure public access to scientific information.

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Laboratory methods to improve SELDI peak detection and quantitation

Jul 02 2007
By Rollin, Dominique ; Whistler, Toni ; Vernon, Suzanne D
Source: Proteome Sci. 2007; 5:9.

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Details:

Alternative Title:

Proteome Sci
Personal Author:

Rollin, Dominique ; Whistler, Toni ; Vernon, Suzanne D

Rollin, Dominique ; Whistler, Toni ; Vernon, Suzanne D Less -
Description:

Background

Protein profiling with surface-enhanced laser desorption-ionisation time-of-flight mass spectrometry (SELDI-TOF MS) is a promising approach for biomarker discovery. Some candidate biomarkers have been identified using SELDI-TOF, but validation of these can be challenging because of technical parameters that effect reproducibility. Here we describe steps to improve the reproducibility of peak detection.

Methods

SELDI-TOF mass spectrometry was performed using a system manufactured by Ciphergen Biosystems along with their ProteinChip System. Serum from 10 donors was pooled and used for all experiments. Serum was fractionated with Expression Difference Mapping kit-Serum Fractionation from the same company and applied to three different ProteinChips. The fractionations were run over a one month period to examine the contribution of sample batch and time to peak detection variability. Spectra were processed and peaks detected using the Ciphergen Express software and variance measured.

Results

Experimental parameters specific to the serum fraction and ProteinChip, including spot protocols (laser intensity and detector sensitivity) were optimized to decrease peak detection variance. Optimal instrument settings, regular calibration along with controlled sample handling and processing nearly doubled the number of peaks detected and decreased intensity variance.

Conclusion

This report assesses the variation across fractionated sera processed over a one-month period. The optimizations reported decreased the variance and increased the number of peaks detected.
Subjects:

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Methodology
Source:

Proteome Sci. 2007; 5:9.
Document Type:

Journal Article
Volume:

5
Collection(s):

CDC Public Access
Main Document Checksum:

[+]

urn:sha256:a48cd197b7a849f85ddb96212eb0d1abaf362b6ab18819b37d1ab0522443c1e0
Download URL:

https://stacks.cdc.gov/view/cdc/3559/cdc_3559_DS1.pdf
File Type:

[PDF-248.75 KB]

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