The Fordyce Lab

uPIC-M: efficient and scalable preparation of clonal single mutant libraries for high-throughput protein biochemistry.

Appel, M.J., Longwell, S.A., Morri, M., Neff, N., Herschlag, D., & Fordyce, P.M. bioRXiv (2021).

(web) (pdf)

Revealing enzyme functional architecture via high-throughput microfluidic enzyme kinetics.

Markin, C.J.*, Mokhtari, D.A.*, Sunden, F., Appel, M.J., Akiva, E., Longwell, S.A., Sabatti, C., Herschlag, D.‡, & Fordyce, P.M.‡, Science (2021). (web) (pdf)

• Science Perspective by Baumer & Whitehead.
• Discussion in Nature.
• Stanford News article.
• Chemical & Engineering News article.

Structure-activity mapping of the peptide- and force-dependent landscape of T-cell activation

Feng, Y., Zhao, X., White, A.K., Garcia, K.C., & Fordyce, P.M., bioRxiv (2021).

(web) (pdf)

Fundamentals to function: quantitative and scalable approaches for measuring protein stability.

Atsavapranee, B.*, Stark, C.D.*, Sunden, S., Thompson, S.‡, & Fordyce, P.M.‡. Cell Systems (2021).

(web) (pdf)

MRBLE-pep measurements reveal accurate binding affinities for B56, a PP2A regulatory subunit.

Hein, J.B., Cyert, M.S., & Fordyce, P.M. ACS Measurement Science (in press).

(web) (pdf)