Amplify 发表于 2025-3-25 04:27:29

https://doi.org/10.1007/978-3-642-51175-2en coordinating homologous recombination events. Here, we describe the use of TFOs such as peptide nucleic acids for targeted genome modification. We discuss this method and its applications and describe protocols for TFO design, delivery, and evaluation of activity in vitro and in vivo.

地壳 发表于 2025-3-25 07:52:31

https://doi.org/10.1007/978-3-642-51175-2eir secondary structure when isolated from the host protein, stapled peptides incorporate an all-hydrocarbon “staple” that reinforces their natural alpha-helical structure. Thus, stapled peptides retain their functional ability to bind their native protein targets and serve multiple experimental use

subacute 发表于 2025-3-25 15:15:08

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Compass 发表于 2025-3-25 19:49:31

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Laconic 发表于 2025-3-25 20:23:12

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事物的方面 发表于 2025-3-26 01:28:57

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arterioles 发表于 2025-3-26 07:23:25

Marcel Mechali,Anne-Marie de Recondosponse to therapy, or to serve as therapeutic targets (Chapman et al., Ann Oncol 18(5):868–873, 2007; Soussi et al., Cancer Res 60:1777–1788, 2000; Anderson and LaBaer, J Proteome Res 4:1123–1133, 2005; Levenson, Biochim Biophy Acta 1770:847–856, 2007). In cancer endogenous levels of protein express

漂泊 发表于 2025-3-26 10:07:57

https://doi.org/10.1007/978-3-319-70211-7ransgenic mouse models, coupled with mass spectrometry proteomics, have served as valuable platform for elucidating the in vivo function of individual genes and proteins. Here we discuss the methods we have recently employed to characterize protein–protein interactions and posttranslational modifica

消极词汇 发表于 2025-3-26 13:19:50

https://doi.org/10.1007/978-3-319-70211-7, soluble in the cytosol or associated to cellular membranes. Importantly, their membrane-inserted form is the main responsible for their apoptotic function. Unfortunately, there are only a limited number of methods available to study the membrane activity of these proteins. Here, we present a metho

下船 发表于 2025-3-26 19:23:56

New Approaches in Intelligent Controlification arise when proteins are of low abundance or are unstable resulting in low yields or poor in vitro activity. In this protocol we describe a method to purify active, recombinant human proteins fused to a tandem MBP tag after expression in human 293T cells.
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