Gök Elmas, Olgaz Seda
Department of Chemistry, Hacettepe University, 06532 Ankara, Turkey.
J Fluoresc. 2004 Mar;14(2):203-6. doi: 10.1023/b:jofl.0000016292.00622.25.
The determination of the fluorophore to the protein molar ratio has been studied using fluorescence spectroscopy. The tyrosine fluorescence is measured from insulin (Ins) solutions at wavelengths lambda(ex)/lambda(em) = 276/300 nm and from fluorescein isothiocyanate (FITC) solutions at lambda(em)/lambda(em) = 494/518 nm. Series of solutions prepared from insulin and FITC are tested for conjugation, recording their fluorimetric intensities. Fluorimetric titrations with different formal concentrations are followed either by intrinsic and extrinsic emission intensities at lambda(ex)/lambda(em) = 276 or 494/518 nm and by their typical emission spectra at pH 9.0. All results denoted a binding ratio of 3 moles of FITC/mole of Ins.
已使用荧光光谱法研究了荧光团与蛋白质的摩尔比。在λ(ex)/λ(em)=276/300 nm波长下测量胰岛素(Ins)溶液的酪氨酸荧光,在λ(em)/λ(em)=494/518 nm波长下测量异硫氰酸荧光素(FITC)溶液的荧光。测试由胰岛素和FITC制备的一系列溶液的缀合情况,记录其荧光强度。用不同的形式浓度进行荧光滴定,随后在λ(ex)/λ(em)=276或494/518 nm处测量内在和外在发射强度,并在pH 9.0下测量其典型发射光谱。所有结果表明FITC与Ins的结合比为3摩尔FITC/摩尔Ins。
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