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Titlebook: Calpain; Methods and Protocol Jeannette S. Messer Book 2019 Springer Science+Business Media, LLC, part of Springer Nature 2019 proteases.en

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Techniques for Imaging with mIBG,sile bond. As with most proteases, they mainly cut unstructured or extended regions of their target proteins. The tendency for concentrated calpain to rapidly autoproteolyze when activated by calcium complicates the kinetic assessment of calpain activity. As calpain autoproteolyzes, the amount of fu
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Case Studies with Abnormal Uptake of mIBG,lated in pathological conditions. Some are ubiquitously expressed (CAPN1, CAPN2, CAPN4, CAPN5, CAPN7, and CAPN10), but others are thought to be localized in specific tissues. The monitoring of in vivo calpain activity is required for physiological, pathological, and therapeutic evaluations. This pas
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,Mechanism of Action of α-Methyl-Dopa,pite the fact that Calpains have been identified in the . genome, their expression patterns and role have not been characterized. Therefore, herein, we describe two methods to determine temporal and spatial expression of Calpain 2 during . development, namely, RT-PCR and whole-mount in situ hybridiz
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https://doi.org/10.1007/978-3-319-24639-0s cytosol-enriched fractions for measuring calpain activity with the fluorogenic substrate N-LY-AMC. With this method one can measure calpain A activity in wild-type flies and in several mutant fly backgrounds, revealing a strong correlation between in situ membrane distribution and in vitro determi
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