Abstract

SummaryPlants must switch rapidly between light harvesting and photoprotection in response to environmental fluctuations in light intensity. This switch can lead to losses in absorbed energy usage, as photoprotective energy dissipation mechanisms can take minutes to hours to fully relax. One possible way to improve photosynthesis is to engineer these energy dissipation mechanisms (measured as non‐photochemical quenching of chlorophyll a fluorescence, NPQ) to induce and relax more quickly, resulting in smaller losses under dynamic light conditions. Previous studies aimed at understanding the enzymes involved in the regulation of NPQ have relied primarily on labor‐intensive and time‐consuming generation of stable transgenic lines and mutant populations – approaches limited to organisms amenable to genetic manipulation and mapping. To enable rapid functional testing of NPQ‐related genes from diverse organisms, we performed Agrobacterium tumefaciens‐mediated transient expression assays in Nicotiana benthamiana to test if NPQ kinetics could be modified in fully expanded leaves. By expressing Arabidopsis thaliana genes known to be involved in NPQ, we confirmed the viability of this method for studying dynamic photosynthetic processes. Subsequently, we used naturally occurring variation in photosystem II subunit S, a modulator of NPQ in plants, to explore how differences in amino acid sequence affect NPQ capacity and kinetics. Finally, we functionally characterized four predicted carotenoid biosynthesis genes from the marine algae Nannochloropsis oceanica and Thalassiosira pseudonana and examined the effect of their expression on NPQ in N. benthamiana. This method offers a powerful alternative to traditional gene characterization methods by providing a fast and easy platform for assessing gene function in planta.

Highlights

  • Conservative projections of population growth have indicated that by 2050 the world’s population will exceed 9.2 billion (Raftery et al, 2012)

  • AtPSBS, AtVDE, and AtZEP are known to play vital roles in non-photochemical quenching of chlorophyll a fluorescence (NPQ) in Arabidopsis. We expressed these genes in fully expanded N. benthamiana leaves using A. tumefaciens-mediated delivery and observed effects on NPQ that were consistent with results observed in stable transgenics of Arabidopsis and other higher plants (Li et al, 2002c; Chen and Gallie, 2012)

  • The increase in zeaxanthin formation did not translate into enhanced NPQ (Figure 4a) as previously observed in stable A. thaliana lines expressing AtCHYB (Johnson et al, 2008). In contrast to this earlier study that showed NPQ levels depend on the de-epoxidation state (DES) of the xanthophyll cycle pool, we found that DES was not an accurate predictor of NPQ in N. benthamiana leaf spots expressing NoCYP97F5

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Summary

SUMMARY

Plants must switch rapidly between light harvesting and photoprotection in response to environmental fluctuations in light intensity. This switch can lead to losses in absorbed energy usage, as photoprotective energy dissipation mechanisms can take minutes to hours to fully relax. We functionally characterized four predicted carotenoid biosynthesis genes from the marine algae Nannochloropsis oceanica and Thalassiosira pseudonana and examined the effect of their expression on NPQ in N. benthamiana. This method offers a powerful alternative to traditional gene characterization methods by providing a fast and easy platform for assessing gene function in planta

INTRODUCTION
RESULTS AND DISCUSSION
CONCLUSIONS
EXPERIMENTAL PROCEDURES
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