Abstract

The issue of whether one or both branches of electron-transfer cofactors is active in Photosystem I (PS I) was studied using a strategy employing interposon mutagenesis and electron paramagnetic resonance (EPR) spectroscopy. PS I complexes were isolated using n-dodecyl-β-d-maltoside (DM) or Triton X-100 (TX-100) from wild-type and mutant strains of Synechococcus sp. PCC 7002 lacking specific PS I polypeptides. The principal values of the g-tensor of A1 were determined by Q-band (34.0 GHz) EPR spectroscopy of perdeuterated, wild-type PS I complexes as gxx = 2.0062, gyy = 2.0050, and gzz = 2.0021, and a stoichiometry of ≤1.0 A1- per P700+ was measured by spin quantitation of photoaccumulated, wild-type PS I complexes at illumination temperatures between 195 and 220 K. The characteristic anisotropic EPR spectrum of A1- was photoaccumulated in all mutant PS I complexes isolated with DM and most mutant PS I complexes isolated with TX-100; however, A0- was photoaccumulated in PS I complexes isolated with TX-100 from the psaF and psaE psaF mutants. PS I complexes isolated with TX-100 from the wild type and the psaE psaF mutant retained 2.5 phylloquinone (PhQ) and 2.6 PhQ per 100 Chl, respectively, indicating that the failure to observe A1- in the psaE psaF mutant is not due to the loss of PhQ. Steady-state rates of light-induced flavodoxin reduction for PS I complexes isolated with DM and TX-100 from the psaF and psaE psaF mutants were nearly identical and differed by less than a factor of 2 from that for the wild-type. The inability to photoaccumulate a second A1- in the wild-type and the psaE psaF mutant indicates that only one of the two resident PhQs in PS I is redox active. The presence of A0- in the psaE and psaE psaF mutants is explained by the protonation and secondary reduction of the semiquinone anion radical of PhQ which is made solvent-accessible by removal of the PsaF polypeptide and by exposure to TX-100. Since only the loss of the C3-distal PsaF or PsaE and PsaF polypeptides affects the spectroscopic properties of A1, the binding site of the redox-active PhQ is associated with the nonprimed α-helices assigned to PsaA/PsaB the electron density map.