Cluster FLISA-A Method to Compare Protein Expression Efficiency Between Cell Lines and Subunit Clustering of Proteins.
Sabrina Brockmöller, Lara Maria Molitor
Abstract
Open AccessNowadays, recombinant proteins are the focus of various research fields, and their use ranges from therapeutic investigations to cellular model systems for the development of therapeutic approaches. Cell systems used for the expression of recombinant proteins should be comparable in terms of yield and expression efficiency. In many research fields, it is desirable to obtain high protein concentrations. A method that combines an easy workflow with rapid results and affordable costs remains missing, and a standardized approach to determining protein concentration in transgenic cell lines is essential for more reliable data analysis. Our protocol demonstrates the cluster fluorescence-linked immunosorbent assay (FLISA), a technique that allows the exact quantification of comparable protein expression amounts. Moreover, it enables the detection of clustered or bound subunits of a protein without necessitating ultracentrifugation. In the present protocol, we demonstrate the utilization of two transgene cell lines, each expressing distinct recombinant proteins, to provide comparability of protein yields and detectable subunit clustering. Key features • Fast and cost-effective approach to integrate into laboratory practice. • Different transgene cell lines are comparable regarding their transgene protein expression yields. • Detection of clustering for up to four different subunits. • Detection of precise antibody concentration for every protein subunit.