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Abscisic acid‐triggered guard cell <scp>l</scp>‐cysteine <i>desulfhydrase</i> function and in situ hydrogen sulfide production contributes to heme oxygenase‐modulated stomatal closure

76

Citations

40

References

2019

Year

Abstract

Recent studies have demonstrated that hydrogen sulfide (H<sub>2</sub> S) produced through the activity of l-cysteine desulfhydrase (DES1) is an important gaseous signaling molecule in plants that could participate in abscisic acid (ABA)-induced stomatal closure. However, the coupling of the DES1/H<sub>2</sub> S signaling pathways to guard cell movement has not been thoroughly elucidated. The results presented here provide genetic evidence for a physiologically relevant signaling pathway that governs guard cell in situ DES1/H<sub>2</sub> S function in stomatal closure. We discovered that ABA-activated DES1 produces H<sub>2</sub> S in guard cells. The impaired guard cell ABA phenotype of the des1 mutant can be fully complemented when DES1/H<sub>2</sub> S function has been specifically rescued in guard cells and epidermal cells, but not mesophyll cells. This research further characterized DES1/H<sub>2</sub> S function in the regulation of LONG HYPOCOTYL1 (HY1, a member of the heme oxygenase family) signaling. ABA-induced DES1 expression and H<sub>2</sub> S production are hyper-activated in the hy1 mutant, both of which can be fully abolished by the addition of H<sub>2</sub> S scavenger. Impaired guard cell ABA phenotype of des1/hy1 can be restored by H<sub>2</sub> S donors. Taken together, this research indicated that guard cell in situ DES1 function is involved in ABA-induced stomatal closure, which also acts as a pivotal hub in regulating HY1 signaling.

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