AI Article Synopsis

  • Mannose-binding lectin (MBL) plays a crucial role in the immune response by activating the complement system and influencing various diseases, including brain ischemia and infections.
  • Developing a new nanoplasmonic assay to detect MBL levels in human serum quickly and efficiently, this method utilizes gold nanorods functionalized with mannose for enhanced detection capabilities.
  • The assay demonstrates high sensitivity and specificity, allowing MBL detection as low as 160 ng/mL in just 15 minutes, paving the way for rapid diagnostics and monitoring in clinical settings.

Article Abstract

Mannose-binding lectin (MBL) activates the complement system lectin pathway and subsequent inflammatory mechanisms. The incidence and outcome of many human diseases, such as brain ischemia and infections, are associated with and influenced by the activity and serum concentrations of MBL in body fluids. To quantify MBL levels, tests based on ELISA are used, requiring several incubation and washing steps and lengthy turnaround times. Here, we aimed to develop a nanoplasmonic assay for direct MBL detection in human serum at the point of care. Our assay is based on gold nanorods (GNRs) functionalized with mannose (Man-GNRs) an amphiphilic linker. We experimentally determined the effective amount of sugar linked to the nanorods' surface, resulting in an approximate grafting density of 4 molecules per nm, and an average number of 11 to 13 MBL molecules binding to a single nanoparticle. The optimal Man-GNRs concentration to achieve the highest sensitivity in MBL detection was 15 μg·mL. The specificity of the assay for MBL detection both in simple buffer and in complex pooled human sera was confirmed. Our label-free biosensor is able to detect MBL concentrations as low as 160 ng·mL within 15 min directly in human serum a one-step reaction and by using a microplate reader. Hence, it forms the basis for a fast, noninvasive, point-of-care assay for diagnostic indications and monitoring of disease and therapy.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC11181273PMC
http://dx.doi.org/10.1021/acsami.4c04018DOI Listing

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