Amino acids in the N-terminal region regulate the photocycle of photoactive yellow protein

The spectroscopic properties of photoactive yellow protein (PYP) partially digested by chymotrypsin were studied. Chymotrypsin yielded three major products that were yellow but distinguishable by SDS-PAGE, They were readily separated by DEAE-Sepharose column chromatography, Protein sequencing and mass spectrometry demonstrated that chymotrypsin cleaved the N-terminal 6, 15, or 23 amino acids (T6, T15, and T23), The blue-shifts of the absorption ma;bma and the increases in the apparent pK(a) of the chromophores relative to those of intact PYP were less than 4 nm and 0,2, respectively, The absorption spectra of the near-UV intermediates produced from T6, T15, and T23 were identical to that of intact PYP, but with lifetimes that were 140, 2,300, and 4,500 times longer, respectively. These observations suggest that the recovery of the dark state of PYP from the near-UV intermediate is accelerated by the N-terminal region, and that this region acts as a regulatory factor for the photocycle of PYP.