4.4 Article

Peridinin chlorophyll a protein:: Relating structure and steady-state spectroscopy

Journal

BIOCHEMISTRY
Volume 39, Issue 17, Pages 5184-5195

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/bi992427s

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Peridinin chlorophyll a protein (PCP) from Amphidinium carterae has been studied using absorbance (OD), linear dichroism (LD), circular dichroism (CD), fluorescence emission, fluorescence anisotropy, fluorescence line narrowing (FLN), and triplet-minus-singlet spectroscopy (T-S) at different temperatures (4-293 K), Monomeric PCP binds eight peridinins and two Chls a. The trimeric structure of PCP, resolved at 2 Angstrom [Hofmann et al. (1996) Science 27, 1788-1791], allows modeling of the Chl a-protein and Chl a-Chl a interactions. The FLN spectrum shows that Chl a is not or is very weakly hydrogen-bonded and that the central magnesium of the emitting Chl a is monoligated. Simulation of the temperature dependence of the absorption spectra indicates that the Huang-Rhys factor, characterizing the electron-phonon coupling strength, has a value of similar to 1. The width of the inhomogeneous distribution function is estimated to be 160 cm(-1). LD experiments show that the two Chls a in PCP are essentially isoenergetic at room temperature and that a substantial amount of PCP is in a trimeric form. From a comparison of the measured and simulated CD, it is concluded that the interaction energy between the two Chls a within one monomer is very weak, <10 cm(-1). In contrast, the Chls a appear to be strongly coupled to the peridinins. The 65 cm(-1) band that is visible in the low-frequency region of the FLN spectrum might indicate a Chl a-peridinin vibrational mode. The efficiency of Chi a to peridinin triplet excitation energy transfer is similar to 100%. On the basis of T-S, CD, LD, and OD spectra, a tentative assignment of the peridinin absorption bands has been made.

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