Photoinactivation of functional photosystem II and D1-protein synthesis in vivo are independent of the modulation of the photosynthetic apparatus by growth irradiance

Planta - Tập 198 - Trang 300-309 - 1996
Youn-Il Park1, Jan M. Anderson1, Wah Soon Chow1
1CSIRO, Division of Plant Industry and Cooperative Research Centre for Plant Science, Canberra, Australia

Tóm tắt

To investigate whether the in-vivo photoinhibition of photosystem II (PSII) function by excess light is an intrinsic property of PSII, the maximal photochemical efficiency of PSII (Fv/Fm) and the content of functional PSII (measured by repetitive flash yield of oxygen evolution) were determined in leaves of pea (Pisum sativum L.), grown in 50 (low light), 250 (medium light), and 650 (high light) μmol photons·m−2·s−1. The modulation of PSII functionality in vivo was induced in 1.1% CO2 by varying either (i) the duration (0–2 h) of light treatment (fixed at 1800 μmol photons· m−2·s−1) or (ii) irradiance (0–3200 μmol photons·m−2·s−1) at a fixed duration (1 h), after infiltration of leaves with water (control), lincomycin (an inhibitor of chloroplast-encoded protein synthesis), or a combination of lincomycin with nigericin (an uncoupler), through the cut petioles of leaves of 22-to 24-d-old plants. The reciprocity law of irradiance and duration of illumination for PSII function in vivo (Park et al. 1995, Planta 196: 401–411) holds in all differently light-grown peas, demonstrating that inactivation of functional PSII depends on photon exposure (mol photons·m−2), not on the rate of photon absorption. In vivo, PSII acts as an intrinsic “photon counter” and at higher photon exposures is inactivated following absorption of about 3 × 107 photons. There is a functional heterogeneity of PSII in vivo with 25% less-stable PSIIs that are inactivated at low photon exposure, compared to 75% more-stable PSIIs regardless of modulation of the photosynthetic apparatus. We suggest that the less-stable PSIIs represent monomers located in the nonappressed granal margins, while the more-stable PSIIs are dimers located in the appressed grana membrane cores. The capacity for D1-protein synthesis was the same in all the light-acclimated peas and saturated at low light, indicating that D1-protein repair is also an intrinsic property of PSII. This accounts for the low intensity required for recovery of photoinhibition in sun and shade plants which is independent of light-harvesting antennae size or PSII/PSI stoichiometries.

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