An
efficient direct approach to triazole-fused sultams has been
developed. The key step of the proposed strategy is base-mediated
cyclization of sulfonamide-tethered 5-iodo-1,2,3-triazoles which are
readily available via an improved protocol for Cu-catalyzed 1,3-dipolar
cycloaddition. The annulation of the sultam fragment to the triazole
ring proceeds smoothly under transition-metal-free conditions in the
presence of Cs2CO3 in dioxane at 100 °C
and affords fused heterocycles in high yields up to 99%. The favorability
of an SNAr-like mechanism for the cyclization was supported
by DFT calculations. The applicability of the developed procedure
to modification of natural compounds was demonstrated by preparation
of a deoxycholic acid derivative.
The cysteine protease Cathepsin B (CtsB) plays a critical role in multiple signaling pathways, intracellular protein degradation, and processing. Endogenous inhibitors regulate its enzymatic activity, including stefins and other cystatins. Recent data proved that CtsB is implicated in tumor extracellular matrix remodeling, cell invasion, and metastasis: a misbalance between cathepsins and their natural inhibitors is often considered a sign of disease progression. In the present study, we investigated CtsB and stefin A (StfA) expression in renal cell carcinoma (RCC). mRNA analysis unveiled a significant CTSB and STFA increase in RCC tissues compared to adjacent non-cancerogenic tissues and a higher CtsB expression in malignant tumors than in benign renal neoplasms. Further analysis highlighted a positive correlation between CtsB and StfA expression as a function of patient sex, age, tumor size, grade, lymph node invasion, metastasis occurrence, and survival. Alternative overexpression and silencing of CtsB and StfA confirmed the correlation expression between these proteins in human RCC-derived cells through protein analysis and fluorescent microscopy. Finally, the ectopic expression of CtsB and StfA increased RCC cell proliferation. Our data strongly indicated that CtsB and StfA expression play an important role in RCC development by mutually stimulating their expression in RCC progression.
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