4.7 Article

Conditioning saliva for use in a microfluidic biosensor

Journal

LAB ON A CHIP
Volume 8, Issue 11, Pages 1847-1851

Publisher

ROYAL SOC CHEMISTRY
DOI: 10.1039/b811150b

Keywords

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Funding

  1. NSF [DGE0203031]
  2. National Institutes of Dental and Craniofacial Research NIDCR [1UO1 DE14971-01]
  3. Coulter Foundation's Translational Research Partnership
  4. NATIONAL INSTITUTE OF DENTAL &CRANIOFACIAL RESEARCH [U01DE014971] Funding Source: NIH RePORTER

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This report details an approach to saliva conditioning for compatibility of raw patient samples with microfluidic immunoassay components, principally biosensor surfaces susceptible to fouling. Stimulated whole human saliva spiked with a small molecule analyte (phenytoin, 252 Da) was. first depleted of cells, debris and high molecular weight glycoproteins (mucins) using membrane. filtration. This process significantly reduced but did not eliminate fouling of biosensor surfaces exposed to the sample. An H-filter, which separates solutes from mixed samples based on their diffusion in laminar flow, was used to extract the analyte from the remaining large molecular weight species in the filtered saliva sample. Patient samples treated in this way retained 23% of the analyte with 97% and 92% reduction in glycoproteins and proteins, respectively, and resulted in 3.6 times less surface fouling than either untreated or filtered saliva alone. These sample conditioning steps will enable the use of fouling-sensitive detection techniques in future studies using clinical saliva samples.

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