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1 ethanol - water extracts were separated on a normal phase.
2 ransition between a superradiant phase and a normal phase.
3 no noticeable effect on the dynamics in the normal phase.
4 engine operation during driving into ER and normal phases.
5 cteristics of the insulating, superfluid and normal phases.
6 amagnetic normal phase, an antiferromagnetic normal phase, a paramagnetic superradiant phase, and an
7 triggered by a quench from the superfluid to normal phase across the Berezinskii-Kosterlitz-Thouless
8 he products were isolated and subjected to a normal-phase amino HPLC for further separation, purifica
9 ur quantum phases, including: a paramagnetic normal phase, an antiferromagnetic normal phase, a param
12 mu(opt) (mm/s) values of 4.10 and 5.22 under normal-phase and 3.74 and 4.34 under reversed-phase elut
14 of AD white matter combining size-exclusion, normal phase, and gas chromatography, immunoassays, and
17 can be retained and quantified under aqueous normal phase (ANP) conditions, using a Diamond Hydride (
18 phic platforms: reversed phase (RP), aqueous normal phase (ANP), and hydrophilic interaction (HILIC)
24 The method utilizes both ion exchange and normal phase chromatography to generate fractions of sat
25 -inducing factors from M. tuberculosis using normal phase chromatography, as well as the use of purif
26 cases, the diastereomers are separable using normal phase chromatography, often resulting in previous
29 LC conditions to separate the tocopherols by normal-phase chromatography and carotenoids by reverse-p
30 sis thaliana glycoproteins were separated by normal-phase chromatography and subsequently identified
35 irconia columns exhibit high stability under normal-phase conditions at relatively high linear veloci
36 mers under reversed-phase, polar organic and normal-phase conditions, demonstrating the versatility o
37 g balance present in the model underlies the normal phase-constant behavior of the swimmeret system.
44 esh tissues were homogenized and analyzed by normal phase high-performance liquid chromatography (HPL
45 t PPARgamma1 activity were fractionated with normal phase high-performance liquid chromatography (NP-
46 d with anthranilic acid, and fractionated by normal phase high-performance liquid chromatography (NP-
48 derivatives that can be separated by silica normal-phase high-performance liquid chromatography (HPL
49 r metabolites in the sera were quantified by normal-phase high-performance liquid chromatography (HPL
50 to separate ceramides and sphingoid bases by normal-phase high-performance liquid chromatography and
53 AC) prior to analysis by either reversed- or normal-phase high-performance liquid chromatography.
54 pids were fractionated into three classes by normal-phase high-performance liquid chromatography.
55 bel oligosaccharides prior to analysis using normal-phase high-performance liquid chromatography.
56 , the method is based on PLOOH separation by normal-phase high-performance thin-layer chromatography,
57 ed between the zone eluting interface (after normal-phase high-performance thin-layer chromatography-
62 c two-phase system and analyzed by isocratic normal-phase HPLC after dissolving the dried sample in t
63 ation of 13(S)-HODE was achieved by use of a normal-phase HPLC and a solvent system containing hexane
69 an mixtures using a combination of capillary normal-phase HPLC coupled off-line to matrix-assisted la
70 protein: a "polar" lipid chromatographing on normal-phase HPLC just before omega-hydroxy ceramide and
75 The synthetic procyanidins are identical by normal-phase HPLC with fractions isolated from cocoa.
77 ce liquid chromatography (HPLC), reverse- or normal-phase HPLC, and capillary electrophoresis (CE) of
78 try, exoglycosidase sequencing combined with normal-phase HPLC, and two-dimensional HPLC mapping.
79 ion due to sample matrix interference in the normal-phase HPLC-APPI-MS/MS system was monitored by the
84 im of this work was to develop an untargeted normal phase LC-MS method, starting from a targeted meth
87 In this work, we compared APPI and APCI for normal-phase LC/MS chiral analysis of five pharmaceutica
88 went solid phase extraction with analysis by normal phase liquid chromatography (LC) with ion trap ma
91 activity of the synthetic [10-(3)H]JHs using normal phase liquid chromatography optimized to give nea
92 al linkage by microanalyzing ceramides using normal phase liquid chromatography-electrospray ionizati
93 rophilic interaction chromatography (HILIC), normal-phase liquid chromatography (NPLC), and supercrit
94 rified fraction of each vegetable oil, using normal-phase liquid chromatography, is described and the
95 ows >95% recovery of LPA, followed by online normal-phase liquid chromatography-mass spectrometry.
96 ature of its putative composite fermion (CF) normal phase, little is known regarding its thermodynami
100 on caused by long bioassay incubation on the normal-phase (NP) plate, zone fixation ((fix)) was achie
101 etection for lipid standards separated using normal-phase (NP)-TLC and NP-HPTLC were established.
104 rticipants could broadly be categorised into normal phase or reversed-phase high performance liquid c
106 ity-but cell position was decoupled from the normal phasing pattern underlying flexion and extension.
107 The oligosaccharide purification uses a normal-phase polyamide resin (DPA-6S) in custom-made pip
109 as speed, practical use of longer columns, a normal-phase retention mechanism, and reduced use of org
112 retical plates/meter for glycocholic acid in normal-phase separation) were preserved in the coupling
113 challenges a Fermi liquid description of the normal phase, shedding new light on the nature of the st
114 l (Hydrastis canadensis) root separated on a normal phase silica gel 60 F(254S) plate and peptides fr
117 rformance liquid chromatography method using normal-phase solvents, a silica column, and evaporative
118 eparative chromatographies (size exclusion + normal phase), target SPME-GC-MS analysis of the hydroly
120 the signature of a first-order superfluid-to-normal phase transition, and disappears at a tricritical
122 two-step process, unveiling an intermediate normal phase with spontaneously broken time-reversal sym