4.4 Article

Variation in LOV Photoreceptor Activation Dynamics Probed by Time-Resolved Infrared Spectroscopy

Journal

BIOCHEMISTRY
Volume 57, Issue 5, Pages 620-630

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/acs.biochem.7b01040

Keywords

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Funding

  1. IMSD-MERGE Program at Stony Brook University [5R25GM103962-04]
  2. Fulbright Program
  3. NSF REU program at Stony Brook University [NSF-CHE-1358959]
  4. OTKA [NN113090]
  5. National Institutes of Health Chemistry-Biology Interface training grant [T32GM092714]
  6. National Science Foundation (NSF) [CHE-1223819]
  7. EPSRC [EP/G002916]

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The light, oxygen, voltage (LOV) domain proteins are blue light photoreceptors that utilize a non-covalently bound flavin mononucleotide (FMN) cofactor as the chromophore. The modular nature of these proteins has led to their wide adoption in the emerging fields of optogenetics and optobiology, where the LOV domain has been fused to a variety of output domains leading to novel light-controlled applications. In this work, we extend our studies of the subpicosecond to several hundred microsecond transient infrared spectroscopy of the isolated LOV domain AsLOV2 to three full-length photoreceptors in which the LOV domain is fused to an output domain: the LOV-STAS protein, YtvA, the LOV-HTH transcription factor, EL222, and the LOV-histidine kinase, LovK Despite differences in tertiary structure, the overall pathway leading to cysteine adduct formation from the FMN triplet state is highly conserved, although there are slight variations in rate. However, significant differences are observed in the vibrational spectra and kinetics after adduct formation, which are directly linked to the specific output function of the LOV domain. While the rate of adduct formation varies by only 3.6-fold among the proteins, the subsequent large-scale structural changes in the full-length LOV photoreceptors occur over the micro- to submillisecond time scales and vary by orders of magnitude depending on the different output function of each LOV domain.

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