AI Article Synopsis

  • Analytical assessment of structural stability and integrity is crucial in developing therapeutic proteins, as it impacts drug efficacy and patient safety.
  • The study introduces a new method, Taylor dispersion analysis (TDA) with LED-UV fluorescence detection, which measures changes in protein size and intrinsic fluorescence during denaturation.
  • This method was used to evaluate the stability of therapeutic proteins like adalimumab and human serum albumin, showcasing a simple process that requires minimal sample size, making it suitable for early drug development stages.

Article Abstract

In the development of therapeutic proteins, analytical assessment of structural stability and integrity constitutes an important activity, as protein stability and integrity influence drug efficacy, and ultimately patient safety. Existing analytical methodologies solely rely on relative changes in optical properties such as fluorescence or scattering upon thermal or chemical perturbation. Here, we present an absolute analytical method for assessing protein stability, structure, and unfolding utilizing Taylor dispersion analysis (TDA) and LED-UV fluorescence detection. The developed TDA method measures the change in size (hydrodynamic radius) and intrinsic fluorescence of a protein during in-line denaturation with guanidinium hydrochloride (GuHCl). The conformational stability of the therapeutic antibody adalimumab and human serum albumin were characterized as a function of pH. The simple workflow and low sample consumption (40 ng protein per data point) of the methodology make it ideal for assessing protein characteristics related to stability in early drug development or when having a scarce amount of sample available.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC9027858PMC
http://dx.doi.org/10.3390/molecules27082506DOI Listing

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