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1 lt to identify the charge variants in a cIEF electropherogram.
2  diagonal in a reconstructed two-dimensional electropherogram.
3 rate spots that fall off the diagonal in the electropherogram.
4 dard deviation of under 5% for the total ion electropherogram.
5 surface was fit to a set of 20 spots in each electropherogram.
6  electropherogram to generate a contour plot electropherogram.
7 g 40% relative standard deviation across the electropherogram.
8 d producing the equivalent of a conventional electropherogram.
9  of 0.28 in the conventional one-dimensional electropherogram.
10  spectra of each of the eluting peaks in the electropherogram.
11  antibody charge variants observed in a cIEF electropherogram.
12 were calculated from their peak areas in the electropherogram.
13 sing peak areas generated from extracted ion electropherograms.
14 exes with DNA, giving distorted peaks in the electropherograms.
15 imaging system are converted to conventional electropherograms.
16 y separated experimentally in the form of an electropherogram, achieving a separation resolution of 1
17  tetrapeptide was obtained directly from the electropherogram and used in the calculation of the DNA-
18                            By overlaying the electropherograms and by performing multivariate analysi
19    Historically, SHAPE data was collected on electropherograms and change in structure was evaluated
20 to deconvolute the components present in the electropherograms and classify the quinoa varieties acco
21 ontactless conductivity detection (CE-C(4)D) electropherograms and interference-free electrospray ion
22 in silico by using computer-simulated NECEEM electropherograms and then applied it to experimental de
23 ts the data quality and repeatability of the electropherograms, and we demonstrate an automatic hando
24                                          The electropherograms appeared in order of anionic content a
25 entified in eight parallel channels when the electropherograms are compared with that of the standard
26 y axes should be changed when the time scale electropherograms are modified to get the distributions.
27                   Within a single injection, electropherograms are obtained for each element of inter
28                                  Single-cell electropherograms are reproducible, with a large number
29  affinity to these motifs is observed in the electropherograms as a change in peak width, which when
30 samples were found to produce representative electropherograms as a single hand-dissected brain sampl
31 semiautomatic procedure for quantitating gel electropherogram-autoradiographs.
32         Compared with visual analysis of the electropherograms, basecaller software frequently missed
33 lecules should generate very narrow peaks in electropherograms, because longitudinal diffusion was th
34 ous identification of all DNA species in the electropherogram, both single- and double-stranded.
35 obility of each DNA extension product in the electropherogram coded the SNPs without the use of a siz
36              In digitonin-treated cells, the electropherograms consisted of a prominent fluorescent p
37                A two-dimensional correlation electropherogram consists of a plot of the correlation i
38                        For signal averaging, electropherograms corresponding to individual pixels can
39 plates, internal/external size standards, or electropherogram data manipulation.
40 erotonin-related analytes from a single-cell electropherogram demonstrates the performance of such a
41                         For each sample, the electropherogram displays a migration time window with a
42 localized to the nucleus was detected on the electropherogram following laser-mediated disruption of
43  comprehensive mathematical model to predict electropherograms for affinity-based separations.
44 ed from beta-Hb is detected in extracted ion electropherograms for glycated beta-Hb.
45               In addition, the corresponding electropherograms for human urine fortified with the tar
46                            The corresponding electropherograms for the standard solution of carnitine
47                   This leads to peaks in the electropherogram from the injection process that are use
48        Statistical analysis of the resulting electropherograms from a population of cells indicated a
49                                Comparison of electropherograms from CE-based denaturing protein analy
50 upole system provided acceptable ion current electropherograms from fmole levels from analytical stan
51                            The time-resolved electropherograms from single and a small group of cereb
52 upole system provided acceptable ion current electropherograms from subpicomole levels of the targete
53 odel is validated by its application for the electropherograms from the diffusion path of a set of pr
54 apillary electrophoresis based on time-scale electropherograms generally uses time-corrected peak are
55                    Moreover, comparison with electropherograms generated from microchip electrophores
56 ber information from standard dye-terminator electropherograms has been little explored, yet this tec
57 s the N-glycan, the peak disappears from the electropherogram, identifying the N-glycan structure.
58 ples analyzed directly, producing a detailed electropherogram in only 120 s on a microfabricated glas
59                            By expressing the electropherogram in terms of signal versus electromigrat
60 unsubstituted rhodamine terminators produced electropherograms in which weak G peaks are observed aft
61 ass detector, all the peaks in the total ion electropherograms, including some totally or partially u
62                                              Electropherograms indicate that the two isomeric forms o
63 oated silica capillary, and the shape of the electropherogram indicated the efficiency is limited by
64                                The resultant electropherograms indicated distinct variations in the c
65  much more relevant to change the time-scale electropherograms into mass relative distribution of the
66 o-dimensional correlation CE, a conventional electropherogram is spread into two dimensions through c
67 to measure and analyze autoradiograms of gel electropherograms is described.
68 encing cause background noise in fluorescent electropherograms, leading to errors in sequence determi
69 e migration order and spacing of peaks in CE electropherograms measured under the same conditions.
70                      Lithophane forms of gel electropherograms, micrographs, electronic and mass spec
71                      On the basis of the 1 D electropherograms obtained, areas supposed to contain th
72 reactions and for peak identification in the electropherogram of an unresolved mixture.
73                              To simplify the electropherogram of clipped forms, the sample is treated
74 hows the presence of additional peaks in the electropherogram of the cancer patient that could be ass
75  use of this integrated microfluidic device, electropherograms of amino acids from individual Jurkat
76 k attributable to dopamine was identified in electropherograms of brain microdialysate samples obtain
77                                              Electropherograms of samples demonstrated the effect of
78 signed to 52 different peaks recorded in the electropherograms of the serum samples.
79              Using a subset of 126 replicate electropherograms of the six viruses and phage for train
80                              The single-cell electropherogram partially resolved approximately 25 com
81 his combination resulted in the most uniform electropherogram profiles, superior to those produced by
82                  This analysis of sequencing electropherograms provides a simple, easily applied meth
83                                          The electropherograms resolved and quantified free ligand as
84        For the immunoassay, the fluorescence electropherograms reveal that CHES provides the optimal
85                                          Gel electropherograms show that the extracted or "soluble" p
86 n time was between 2 and 3% for selected ion electropherograms (SIEs) generated for six ions; median
87 /reTOFMS combination, resulting in total ion electropherograms similar to those obtained using UV abs
88 ver 60 additional peaks were detected in the electropherograms, suggesting the potential for monitori
89         Monitoring of insulin secretion with electropherograms taken at 15-s intervals resolved secre
90 sfully identify components seen in UV or LIF electropherograms, thereby expanding the capability of C
91      HT detection is performed on each pixel electropherogram to generate a contour plot electrophero
92    This finding was attributed to the use of electropherograms to detect artifacts such as aggregator
93 quired to perform the variable change on the electropherogram was developed with an emphasis on the f
94 d CE separation efficiency for the SIM CE/MS electropherograms was determined to be 2860 plates (peak
95 >90% increase in area under the curve of the electropherograms was observed with the interface compar
96    Additional properties exhibited in the CE electropherograms were also explained using the computer
97                                              Electropherograms were also obtained for purified mammal
98 ragments were precisely sized (+/-1 bp), and electropherograms were generated for each genome with Ge
99                                         When electropherograms were normalized to total protein conte
100 d the monitoring of overlapping peaks in the electropherogram when newly formed products resulting fr
101  B using the new device produced a CE-ESI-MS electropherogram with a signal-to-noise ratio of over 10
102                                              Electropherograms with 100,000 theoretical plates were a
103 time course of release was registered in the electropherograms with subsecond resolution.
104 of the PCR products were determined from the electropherogram without using a calibration plot and cu

 
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