PRIMARY, SECONDARY, TERTIARY, AND Q

PRIMARY, SECONDARY, TERTIARY, AND QUATERNARY STRUCTURE.

Primary Sequence from Cloning The sequence of wild-type Aequorea GFP is given in Figure 1. Sequences of at least four other isoforms are known(19),though none of the mutations seem to be in positions known to influence protein behavior. Most cDNA constructs derivedfromtheoriginalsequencecontaintheinnocuousmutationQ80R,probably resulting from a PCR error (11). Also, the gene has been resynthesized withalteredcodonsandimprovedtranslationalinitiationsequences(seesection on “Promoters, Codon Usage, and Splicing”). The chromophore is a p-hydroxybenzylideneimidazolinone (10,20) formed from residues 65–67, which are Ser-Tyr-Gly in the native protein. Figure 2 shows the currently accepted mechanism (21–23) for chromophore formation. First, GFP folds into a nearly native conformation, then the imidazolinone is formed by nucleophilic attack of the amide of Gly67 on the carbonyl of residue 65, followed by dehydration. Finally, molecular oxygen dehydrogenates the α-β bond of residue 66 to put its aromatic group into conjugation with the imidazolinone. Only at this stage does the chromophore acquire visible absorbance and fluorescence. This mechanism is based on the following arguments: (a) Atmospheric oxygen is required for fluorescence to develop (21,24). (b) Fluorescence of anaerobically preformed GFP develops with a simple exponential time course after air is readmitted (21,25), which is essentially unaffected by the concentration of the GFP itself or of cellular cofactors. (c)Analogousimidazolinonesautoxidizespontaneously(26).(d)Theproposed