Quantification of Protein Markers in Cortical Cells

Deidentified tissue samples were obtained at Stanford University School of Medicine under a protocol approved by the Research Compliance Office at Stanford University. Brain tissue samples at PCWs 20 to 22 were delivered on ice and processed within 3 hours of the procedure. Tissue was processed according to a previously published protocol (89 (link)) to obtain a single-cell suspension. Cells were stained with the following antibodies on ice for 30 min: anti-CD45 (1:25, clone HI30, BioLegend), anti-O4 (1:20, R&D Systems), anti-IGF2R (1:10, BD Biosciences), anti-CD22 (1:20, clone HIB22, BioLegend), anti-MBP (1:100, clone SMI 99, BioLegend), anti-MAP2 (1:20, SMI 52, BioLegend), and human Fc block (1:20, BD Biosciences). After staining, cells were washed, and relevant populations were analyzed on a BD LSRFortessa. Quantibrite–phycoerythrin (PE) (BD Biosciences) beads were resuspended in FACS buffer and analyzed on a BD LSRFortessa. Using the same laser powers and detector voltages, cortical cells and Ramos cells were analyzed for CD22 expression. A standard curve was constructed to correlate PE intensity with number of PE molecules per Quantibrite bead. Last, molecule numbers on human primary cortical brain cell types were calculated by interpolation.

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Pluvinage J.V., Sun J., Claes C., Flynn R.A., Haney M.S., Iram T., Meng X., Lindemann R., Riley N.M., Danhash E., Chadarevian J.P., Tapp E., Gate D., Kondapavulur S., Cobos I., Chetty S., Pașca A.M., Pașca S.P., Berry-Kravis E., Bertozzi C.R., Blurton-Jones M, & Wyss-Coray T. (2021). The CD22-IGF2R interaction is a therapeutic target for microglial lysosome dysfunction in Niemann-Pick type C. Science translational medicine, 13(622), eabg2919.

Publication 2021

anti-O4 human Fc block BD LSRFortessa Quantibrite–phycoerythrin (PE)

Antibodies Brain Buffer Cells Clone Cortical Human Igf2r Map2 Phycoerythrin Populations Tissue

Corresponding Organization : Neurosciences Institute

Other organizations : University of California, Irvine, Harvard University, Boston Children's Hospital, Organogenesis (United States), Howard Hughes Medical Institute, University of California, San Francisco, Rush University Medical Center

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Variable analysis

independent variables

None explicitly mentioned

dependent variables

Expression levels of CD45, O4, IGF2R, CD22, MBP, and MAP2 on cortical brain cells

control variables

Tissue samples were obtained from gestational weeks 20 to 22
Tissue samples were processed within 3 hours of the procedure
Cells were stained with specific antibodies on ice for 30 minutes
Quantibrite-PE beads were used to create a standard curve for correlating PE intensity with number of PE molecules

controls

Positive control: Ramos cells were analyzed for CD22 expression using the same laser powers and detector voltages as the cortical cells
Negative control: Not explicitly mentioned

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