ABSTRACT
The metalloprotein cytochrome c' was extracted and purified from the bacterium Paracoccus denitrificans in order to develop a specific biosensing system for nitric oxide (NO). The metalloprotein was encapsulated in a porous silicate sol-gel glass to enable spectroscopic changes in the haem centre as a function of NO ligation to be quantified using absorption measurements. Spectroscopic evidence suggested that, between 2 and 4 d after encapsulation, the cytochrome c' protein changed conformation in the locality of the haem moiety, possibly from a five to a six coordinate haem centre. Such conformational changes were also observed when the cytochrome c' was stored in solution, although over a 2-3 month period. The conformational changes occurring in the protein altered the spectral characteristics of the reduced, oxidised and nitrosyl complex of the cytochrome c' and appear to change the binding affinity of the protein towards NO. However, the encapsulated (reconformed) cytochrome c' was shown to retain its selectivity towards NO with good reproducibility (seven consecutive measurements of NO produced an intensity value with a relative standard deviation of 0.28%). An NO calibration curve, using the in situ release of NO from the donor diethylamine NONOate, was obtained for the encapsulated cytochrome c' with an approximate working range of 10-400 mumol l-1.
Subject(s)
Nitric Oxide/analysis , Biosensing Techniques , Cytochrome c Group , HumansABSTRACT
Aequorin, the bioluminescent protein found in the jellyfish Aequorea sp., has been immobilized in a porous sol-gel glass environment. The luminescence from this protein is specifically triggered by the presence of calcium ions, thus offering exciting possibilities for the development of an optical biosensor for this cationic species. The luminescence emission spectrum has been measured from the aequorin protein after interaction with calcium ions. The intensity of the luminescence, measured at the peak maximum of 470 nm, for the encapsulated protein has been calibrated against calcium ion concentration. The characterization of the protein within the sol-gel matrix has been reported together with biosensing experiments using human sera and milk samples. The results suggest that the sol-gel encapsulated aequorin protein offers potential as a one shot bioluminescence based biosensor for the determination of calcium ions in such complex matrices.
