TY - JOUR
T1 - Trimethyl-substituted carbamate as a versatile self-immolative linker for fluorescence detection of enzyme reactions
AU - Nakamura, Noriaki
AU - Uchinomiya, Shohei
AU - Inoue, Kazuya
AU - Ojida, Akio
N1 - Funding Information:
Funding: This research was funded by a Grant-in-Aid for Scientific Research on Innovative Areas “Chemistry for Multimolecular Crowding Biosystems” (JSPS KAKENHI Grant No. JP17H06349), Grant-in-Aid for Challenging Exploratory Research (JSPS KAKENHI Grant No. JP17K19203). A.O. acknowledges Naito Science Foundation and Toray Science Foundation for their financial supports.
Funding Information:
This research was funded by a Grant-in-Aid for Scientific Research on Innovative Areas "Chemistry for Multimolecular Crowding Biosystems" (JSPS KAKENHI Grant No. JP17H06349), Grant-in-Aid for Challenging Exploratory Research (JSPS KAKENHI Grant No. JP17K19203). A.O. acknowledges Naito Science Foundation and Toray Science Foundation for their financial supports.
Publisher Copyright:
© 2020 by the authors.
PY - 2020/5
Y1 - 2020/5
N2 - Self-immolative linker is a useful building block of molecular probes, with broad applications in the fields of enzyme activity analysis, stimuli-responsive material science, and drug delivery. This manuscript presents N-methyl dimethyl methyl (i.e., trimethyl) carbamate as a new class of self-immolative linker for the fluorescence detection of enzyme reactions. The trimethyl carbamate was shown to spontaneously undergo intramolecular cyclization upon formation of a carboxylate group, to liberate a fluorophore with the second time rapid reaction kinetics. Interestingly, the auto-cleavage reaction of trimethyl carbamate was also induced by the formation of hydroxyl and amino groups. Fluorescent probes with a trimethyl carbamate could be applicable for fluorescence monitoring of the enzyme reactions catalyzed by esterase, ketoreductase, and aminotransferase, and for fluorescence imaging of intracellular esterase activity in living cells, hence demonstrating the utility of this new class of self-immolative linker.
AB - Self-immolative linker is a useful building block of molecular probes, with broad applications in the fields of enzyme activity analysis, stimuli-responsive material science, and drug delivery. This manuscript presents N-methyl dimethyl methyl (i.e., trimethyl) carbamate as a new class of self-immolative linker for the fluorescence detection of enzyme reactions. The trimethyl carbamate was shown to spontaneously undergo intramolecular cyclization upon formation of a carboxylate group, to liberate a fluorophore with the second time rapid reaction kinetics. Interestingly, the auto-cleavage reaction of trimethyl carbamate was also induced by the formation of hydroxyl and amino groups. Fluorescent probes with a trimethyl carbamate could be applicable for fluorescence monitoring of the enzyme reactions catalyzed by esterase, ketoreductase, and aminotransferase, and for fluorescence imaging of intracellular esterase activity in living cells, hence demonstrating the utility of this new class of self-immolative linker.
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U2 - 10.3390/molecules25092153
DO - 10.3390/molecules25092153
M3 - Article
C2 - 32380657
AN - SCOPUS:85084392726
SN - 1420-3049
VL - 25
JO - Molecules
JF - Molecules
IS - 9
M1 - 2153
ER -