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1 rdinarily cooperative equilibrium folding of simple proteins.
2 ing the factors that govern folding rates of simple proteins.
5 owing field of proteomic research, rapid and simple protein analysis is a crucial component of protei
6 rature jumps in the acid-denatured form of a simple protein and monitored by fluorescence resonance e
7 assay (PLA) is one of the most sensitive and simple protein assays developed to date, yet a major lim
8 nhanced fluorescence (MAMEF), we show that a simple protein-based assay system can be optically ampli
9 rly remarkable are those enzymes that act as simple protein catalysts, without the assistance of meta
11 atory sites is interpreted primarily through simple protein-DNA and protein-protein interactions, wit
13 ding and unfolding kinetics of mutants for a simple protein folding reaction to characterize the stru
14 The rapid evolution of gene products with simple protein folds and a lack of well-characterized fu
19 Residue level analysis of the folding of simple proteins may hold the key to understanding foldin
20 ed to modification analyses of proteins in a simple protein mixture, Cdc2p protein complexes isolated
23 f MSAD for interrogating intact proteins and simple protein mixtures in a multiplexed manner, we have
24 analysis of protein aggregates, as found in simple protein mixtures, to complex aggregates, as found
26 in folding has been studied extensively with simple protein models such as short cubic-lattice chains
27 rk has investigated the energy landscapes of simple protein models, but what do the landscapes of rea
28 cterize the polypeptide molecular weights of simple proteins or glycoproteins or to determine the sto
29 have monitored the folding of a kinetically simple protein, peptostreptococcal protein L (protein L)
33 n that are predictable based on the rules of simple protein-protein and protein-DNA interactions.
35 trast CT allows differentiation of simulated simple, protein-rich, hemorrhagic, and enhancing renal c
36 ro phantom specifically designed to simulate simple, protein-rich, hemorrhagic, and enhancing renal c
38 is no uniformly superior algorithm, and that simple protein similarity measures combined with hierarc
40 el four-stranded coiled coils are relatively simple protein structures that embody a heptad sequence
41 re, we report the development of a small and simple protein tag that complements the therapeutic and
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