Maintenance and Manipulation of Chicken DT40 and Jurkat Cells

Culture maintenance, plasmid transfection and BCR stimulation of chicken DT40 B cell lines were carried out as previously described^{46 (link)}. Jurkat cell culture and transfection techniques were also performed as described^{8 (link)}. The SOS1⁻2⁻deficient DT40 B cells were generated in Dr. Tomohiro Kurosaki’s laboratory (RIKEN). Both wildtype and SOS1⁻2⁻ deficient DT40 B cells were gifts from Dr. Kurosaki. Obtained cell lines were confirmed to be free of mycoplasma contamination. For routine cell functional authentication, surface expression of B cell receptor (BCR) was confirmed by flow cytometry and by BCR-induced pERK2 measurement similar to the experiment shown in Supplementary Figure 4. Jurkat T cells were obtained from ACCC and were maintained according to the provided guideline.
To generate EGFP-tagged hSOS1 variants, EGFP coding sequence (CDS) was PCR-amplified with Xba I- and Not I-flanked primers from pEGFP-N1 plasmid (Clonetech). Resulting SOS1-EGFP construct bears a 5 amino acid linker (SRGGR) between SOS1 and EGFP CDS. Expression was confirmed by Western blotting with anti-GFP antibody (Supplementary Fig. 4a).

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Christensen S.M., Tu H.L., Jun J.E., Alvarez S., Triplet M.G., Iwig J.S., Yadav K.K., Bar-Sagi D., Roose J.P, & Groves J.T. (2016). One-way membrane trafficking of SOS in receptor-triggered Ras activation. Nature structural & molecular biology, 23(9), 838-846.

Publication 2016

pEGFP-N1 plasmid

Amino acid Anti antibody B cell receptor B cells Bears Cell Cell culture Cell lines Cell surface receptor Chicken Coding sequence Flow cytometry Gifts Jurkat cells Mycoplasma Plasmid Primers Transfection

Corresponding Organization :

Other organizations : University of California, Berkeley, University of California, San Francisco, Howard Hughes Medical Institute, New York University

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Variable analysis

independent variables

Culture maintenance
Plasmid transfection
BCR stimulation of chicken DT40 B cell lines
Jurkat cell culture and transfection techniques

dependent variables

Surface expression of B cell receptor (BCR)
BCR-induced pERK2 measurement
Expression of EGFP-tagged hSOS1 variants confirmed by Western blotting with anti-GFP antibody

control variables

Cell lines were confirmed to be free of mycoplasma contamination
Wildtype and SOS1^-2^- deficient DT40 B cells were used as controls

positive controls

Experiment shown in Supplementary Figure 4 for BCR-induced pERK2 measurement

negative controls

Wildtype DT40 B cells

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