High yield of secondary B-side electron transfer in mutant Rhodobacter capsulatus reaction centers

  • Lucas Kressel
  • , Kaitlyn M. Faries
  • , Marc J. Wander
  • , Charles E. Zogzas
  • , Rachel J. Mejdrich
  • , Deborah K. Hanson
  • , Dewey Holten
  • , Philip D. Laible
  • , Christine Kirmaier

Research output: Contribution to journalArticlepeer-review

15 Scopus citations

Abstract

From the crystal structures of reaction centers (RCs) from purple photosynthetic bacteria, two pathways for electron transfer (ET) are apparent but only one pathway (the A side) operates in the native protein-cofactor complex. Partial activation of the B-side pathway has unveiled the true inefficiencies of ET processes on that side in comparison to analogous reactions on the A side. Of significance are the relative rate constants for forward ET and the competing charge recombination reactions. On the B side, these rate constants are nearly equal for the secondary charge-separation step (ET from bacteriopheophytin to quinone), relegating the yield of this process to < 50%. Herein we report efforts to optimize this step. In surveying all possible residues at position 131 in the M subunit, we discovered that when glutamic acid replaces the native valine the efficiency of the secondary ET is nearly two-fold higher than in the wild-type RC. The positive effect of M131 Glu is likely due to formation of a hydrogen bond with the ring V keto group of the B-side bacteriopheophytin leading to stabilization of the charge-separated state involving this cofactor. This change slows charge recombination by roughly a factor of two and affords the improved yield of the desired forward ET to the B-side quinone terminal acceptor.

Original languageEnglish
Pages (from-to)1892-1903
Number of pages12
JournalBiochimica et Biophysica Acta - Bioenergetics
Volume1837
Issue number11
DOIs
StatePublished - Nov 2014

Keywords

  • Charge recombination
  • Directed evolution
  • High-throughput screening
  • Photosynthetic reaction center
  • Transmembrane electron transfer
  • Ultrafast spectroscopy

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