Quantifying KCNB1 Channel Surface Expression

Frozen aliquots of CHO-K1 cells electroporated with WT or variant KCNB1 channels were thawed and grown under the same conditions used for automated patch clamp recording. Cell-surface biotinylation and immunoblotting were performed as previously described^{7 (link),14 (link)}, 60–72h post-electroporation, using mouse anti-K_V2.1 (1:250; K89/34, Antibodies Inc), mouse anti-transferrin receptor (1:500; H68.4, ThermoFisher), and rabbit anti-calnexin (1:250; H70, Santa Cruz Biotechnology), Alexa Fluor 680-goat anti-rabbit IgG (1:20,000, Jackson ImmunoResearch) and Alexa Fluor 790-goat anti-mouse IgG (1:20,000, Jackson ImmunoResearch) antibodies.
Normalized total, surface, and surface/total protein ratio results were derived from 3 independent experiments. Calnexin immunoreactivity was present in total protein lysates and absent from the cell-surface fraction, confirming the selectivity of biotin labeling for cell-surface protein.

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Kang S.K., Vanoye C.G., Misra S.N., Echevarria D.M., Calhoun J.D., O’Connor J.B., Fabre K.L., McKnight D., Demmer L., Goldenberg P., Grote L.E., Thiffault I., Saunders C., Strauss K.A., Torkamani A., van der Smagt J., van Gassen K., Carson R.P., Diaz J., Leon E., Jacher J.E., Hannibal M.C., Litwin J., Friedman N.R., Schreiber A., Lynch B., Poduri A., Marsh E.D., Goldberg E.M., Millichap J.J., George AL J.r, & Kearney J.A. (2019). Spectrum of KV2.1 Dysfunction in KCNB1-associated Neurodevelopmental Disorders. Annals of neurology, 86(6), 899-912.

Publication 2019

Alexa Fluor 680-goat anti-rabbit IgG Alexa Fluor 790-goat anti-mouse IgG

Anti igg Antibodies Biotin Biotinylation Calnexin Cell Cell surface protein Cho cells Electroporation Frozen Goat Mouse Mouse transferrin receptor 1 Protein Rabbit Selectivity Surface protein

Corresponding Organization : Northwestern University

Other organizations : Lurie Children's Hospital, Levine Children's Hospital, Harvard University, Massachusetts General Hospital, Children's Mercy Hospital, University of Missouri–Kansas City, Clinic for Special Children, Scripps Research Institute, University Medical Center Utrecht, Monroe Carell Jr. Children's Hospital, Children's National, University of Michigan–Ann Arbor, University of California, San Francisco, UCSF Benioff Children's Hospital, Cleveland Clinic, Temple Street Children's University Hospital, Boston Children's Hospital, Children's Hospital of Philadelphia

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Variable analysis

independent variables

Transfection of wild-type or variant KCNB1 channels in CHO-K1 cells

dependent variables

Cell-surface expression of KCNB1 channels
Protein levels of KCNB1 channels, transferrin receptor, and calnexin

control variables

Growth conditions for CHO-K1 cells
Time point for analysis (60-72h post-electroporation)

controls

Positive control: Cell-surface biotinylation and immunoblotting for transferrin receptor
Negative control: Absence of calnexin immunoreactivity in the cell-surface fraction, confirming the selectivity of biotin labeling for cell-surface proteins

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