Sandbox122

The structure of a flaving domain, LOV2, from the chimeric phototropin photoreceptor PHY3, has been determined thanks to X-Ray diffraction. This domain is composed by four chains which are identical and called A, B, C and D. It's a L-polypeptide which weight is 50552,99 Da. Each chains has 104 aminoacids and possess four (28 residues which represents 26%) and six B (37 residues which represent 35%).

The (Flavin MonoNucleotide) is the ligand which is responsible for the light absorption. A single molecule of FMN is bound non convalently in the interior of LOV2 domain. FMN is stabilized thanks to hydrogen bonds, Van der Waals and electrostatic interactions. For example, atoms and (alpha C helix) create ionic bond with phosphate group of FMN. , , , (alpha A helix and beta-strand C, D and E) aminoacid make some electrostatic interaction which stabilize FMN. Some results indicate that the majority of the FMN in the LOV2 domain exist in the protonated form. Researcher propose a reaction mechanism that involves excited-state proton transfer, on the nanosecond time scale , from the sulfhydryl group of the conserved cysteine to the N5 atom of FMN. Blue light arrives on the only LOV2 (situate 4.2A from atom C(4a)) and induces formation of covalent cysteinyl-C(4a)adduct. (To explain that, refer to the scheme). Somes studies showed that temperature have an influence on that adduct. In fact, at low temperature, the microenvironment determine the reactivity of the S-H group of . A base-catalyzed mechanism for dark state recovery. Imidazole snatch proton from N5 atom of FMN and give it to the cysteine again (explain on the scheme).

Some studies have showed a role for the central β-sheet in propagating the signal generated within the FMN-protein changes at the LOV2 surface, which are necessary for activation of the C-terminal kinase domain.Specifically, the side chain of a conserved glutamine residue within LOV2 (Gln575 in Arabidopsis phot1) which forms hydrogen bonds with the FMN chromophore flips by 180° upon cysteinyl adduct formation causing protein changes in the central β-sheet that forms contacts with the Jα-helix.

The current view of phototropin receptor activation is that LOV2 functions as a repressor of the C-terminal kinase domain in the dark and that this mode of repression is alleviated upon photoexcitation, resulting in receptor autophosphorylation.The predominant role of LOV2 in regulating phototropin activity appears to arise from its position within the phototropin molecule. Photoexcitation of an extended LOV2 fragment leads to displacement of an α-helix from the surface of the LOV2-core.

Kinase will permit the autophosphorylation of phototropin. The rate of phosphorylatide phototropin acts to differential lateral gradients of auxin which is responsible of phototropism phenomenon. For more information about the continuation of this mechanism refer to this PDB protein: 2z6c,2z6d,

.John T. M. Kennis, Ivo H. M. van Stokkum, Sean Crosson, Magdalena Gauden, Keith Moffat, and Rienk van Grondelle:The LOV2 Domain of Phototropin: A Reversible Photochromic Switch.J. Am. Chem. Soc., 2004, 126 (14), pp 4512–4513.

.Maxime T. A. Alexandre, Jos C. Arents, Rienk van Grondelle, Klaas J. Hellingwerf, and John T. M. Kennis:A Base-Catalyzed Mechanism for Dark State Recovery in the Avena sativa Phototropin-1 LOV2 Domain. Biochemistry, 2007, 46 (11), pp 3129–3137.

.Crosson S, Moffat KStructure of a flavin-binding plant photoreceptor domain: insights into light-mediated signal transductionProc. Natl. Acad. Sci. U. S. A. v98, p.2995-3000.

software used: pymol, chemstek

David Bauché, Romain Daillere