Proteolytic activity monitored by fluorescence resonance energy transfer through quantum-dot–peptide conjugates

被引:0
|
作者
Igor L. Medintz
Aaron R. Clapp
Florence M. Brunel
Theresa Tiefenbrunn
H. Tetsuo Uyeda
Eddie L. Chang
Jeffrey R. Deschamps
Philip E. Dawson
Hedi Mattoussi
机构
[1] Center for Bio/Molecular Science and Engineering,Optical Sciences Division
[2] Code 6900,Departments of Cell Biology & Chemistry and the Skaggs Institute for Chemical Biology
[3] US Naval Research Laboratory,undefined
[4] Code 5611,undefined
[5] US Naval Research Laboratory,undefined
[6] The Scripps Research Institute,undefined
[7] Laboratory for the Structure of Matter,undefined
[8] Code 6030,undefined
[9] US Naval Research Laboratory,undefined
来源
Nature Materials | 2006年 / 5卷
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摘要
Proteases are enzymes that catalyse the breaking of specific peptide bonds in proteins and polypeptides. They are heavily involved in many normal biological processes as well as in diseases, including cancer, stroke and infection. In fact, proteolytic activity is sometimes used as a marker for some cancer types. Here we present luminescent quantum dot (QD) bioconjugates designed to detect proteolytic activity by fluorescence resonance energy transfer. To achieve this, we developed a modular peptide structure which allowed us to attach dye-labelled substrates for the proteases caspase-1, thrombin, collagenase and chymotrypsin to the QD surface. The fluorescence resonance energy transfer efficiency within these nanoassemblies is easily controlled, and proteolytic assays were carried out under both excess enzyme and excess substrate conditions. These assays provide quantitative data including enzymatic velocity, Michaelis–Menten kinetic parameters, and mechanisms of enzymatic inhibition. We also screened a number of inhibitory compounds against the QD–thrombin conjugate. This technology is not limited to sensing proteases, but may be amenable to monitoring other enzymatic modifications.
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页码:581 / 589
页数:8
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