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1 runcated AhRs were also subjected to limited trypsinization.
2 arated from epithelial cells by differential trypsinization.
3 degree of spreading of cells replated after trypsinization.
4 r removal of the drug and further passage by trypsinization.
5 the sialylated region of glycophorin by mild trypsinization.
6 in astrocytes, which was prevented by light trypsinization.
7 isease linked mutants A30P and A53T, by mild trypsinization (0.1%, 30 s) of Ltk(-) cotransfected cell
8 observed extensive RNA degradation following trypsinization, a routine procedure used to dissociate a
14 Beginning with intact spheroids, a serial trypsinization and trituration procedure was used to iso
16 n and spreading, detachment and signaling by trypsinization, and signaling through either epidermal g
18 ment characteristic of the TGN; or (ii) mild trypsinization at neutral pH, resulted in the activation
19 vitro by different external stimuli such as trypsinization, cell density, and serum concentration.
22 er, when the labeled enzyme was subjected to trypsinization, followed by sequencing of the labeled pe
23 ne disruption by depletion of cholesterol or trypsinization halts B(2)R internalization, invasion, an
24 bitors of protein secretion and abolished by trypsinization, indicating that the active substance inc
27 rotomer (Ibp) bound to the cell surface, but trypsinization of Ibp was necessary for docking of the A
31 by secondary structure in the protein, since trypsinization of reduced and carboxymethylated RF-hsp 7
33 posed loop in the GII.3 NoVs facilitates the trypsinization of the capsid protein in the assembled fo
37 remain within the membrane domain following trypsinization of the intact gastric H,K-ATPase in the p
38 steroid binding domain generated by partial trypsinization of the rat uterine ER, we demonstrate tha
41 LP-mediated fusion activity was dependent on trypsinization of VP4, and the strain-specific phenotype
43 has the advantage of reducing the effects of trypsinization on measurements of adhesion, and therefor
51 ts are distinct from those obtained from the trypsinization studies performed earlier on the NV (GI)
53 din-based affinity purification and on-resin trypsinization, the resulting peptide mixture is subject
54 tress fibers were fewer and shorter, and the trypsinization time needed for cells to round up was red
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