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1 T-->A transversion at nucleotide 1796) using restriction enzyme analysis.
2 00 ethnically matched control individuals by restriction enzyme analysis.
3 potentially functional and were confirmed by restriction enzyme analysis.
4 ase chain reaction products was confirmed by restriction enzyme analysis.
5 tained unique ITS alleles distinguishable by restriction enzyme analysis.
6 nd was excluded from 50 unaffected people by restriction enzyme analysis.
7 ific DNA sequences easily distinguishable by restriction enzyme analysis.
8 e confirmed by reverse strand sequencing and restriction enzyme analysis.
9 e between 1997 and 2003 were genome typed by restriction enzyme analysis.
10 transcription-polymerase chain reaction and restriction enzyme analysis.
11 chain reaction (RT-PCR) in combination with restriction enzyme analysis.
12 determined by type-specific PCR followed by restriction enzyme analysis.
13 d mutations in other cases were confirmed by restriction-enzyme analysis.
15 clones were determined to be unique based on restriction enzyme analysis, and 42 of these were found
17 Molecular methods, including karyotyping and restriction enzyme analysis, confirmed that the isolates
18 bination of the heteroduplex tracking assay, restriction enzyme analysis, DNA sequencing, and reverse
19 above method where isoelectric focusing and restriction enzyme analysis failed to identify the natur
22 A extracted using this method lent itself to restriction enzyme analysis, ligation, transformation, a
23 Mycobacterium species were identified by restriction enzyme analysis of a 439-bp segment of the 6
27 , which interrogates DNA methylation via the restriction enzyme analysis of PCR-amplified bisulfite t
30 ncluded growth and biochemical analysis, PCR-restriction enzyme analysis of the 439-bp Telenti fragme
31 uid chromatography, and, when necessary, PCR-restriction enzyme analysis of the 65-kDa heat shock pro
32 isolates matched the ATCC type strain by PCR restriction enzyme analysis of the 65-kDa hsp gene seque
33 s, B. burgdorferi isolates were subjected to restriction enzyme analysis of the amplified ospC genes
34 n of PCR amplification of 16S rRNA genes and restriction enzyme analysis of the amplified products.
35 tudy was to identify Capnocytophaga spp. via restriction enzyme analysis of this gene (16S rRNA PCR-r
36 ation of each virus strain was determined by restriction enzyme analysis of total cellular DNA, by PC
38 nd circulation periods were characterized by restriction enzyme analysis of viral DNA and select gene
40 n of methylation using methylation-sensitive restriction enzyme analysis or focused on single-copy ge
41 sasii isolates from the United States by PCR restriction enzyme analysis (PRA) of the 441-bp Telenti
42 ve group, of which 48 (70%) had the same PCR restriction enzyme analysis (PRA) profile as the hsp65 g
43 On the basis of their susceptibility and restriction enzyme analysis profiles, our findings indic
44 defined by using small-fragment chromosomal restriction-enzyme analysis, pulsed-field gel electropho
45 tests; (ii). molecular techniques involving restriction enzyme analysis (REA) of portions of the 16S
46 polymerase chain reaction (AP-PCR), HindIII restriction enzyme analysis (REA), and pulsed-field gel
47 ile isolates from 102 patients were typed by restriction enzyme analysis (REA), arbitrarily primed PC
58 morphic DNA analysis-based genotyping and by restriction enzyme analysis with enzymes BsmAI and NspBI