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1 nonspecific effect of DNA insertion into the plasmid vector.
2 niquely placed in either strand of a shuttle plasmid vector.
3 1,500 bp were gel purified and cloned into a plasmid vector.
4 ed with the kanamycin resistance gene of the plasmid vector.
5 cDNA copy of BVDV NADL in a low-copy-number plasmid vector.
6 A-mediated type I IFN activation in a single plasmid vector.
7 the output of RDA was shotgun cloned into a plasmid vector.
8 ol of a heterologous inducible promoter on a plasmid vector.
9 produced empty capsids when expressed from a plasmid vector.
10 ed in trans by the rfc gene expressed from a plasmid vector.
11 esis gene BIO6 were introduced together on a plasmid vector.
12 G1a was expressed and purified using a novel plasmid vector.
13 ol, E. coli RecA was expressed from the same plasmid vector.
14 from a pool of PCR products and a linearized plasmid vector.
15 quences of the adeno-associated virus to the plasmid vector.
16 d be restored by reintroduction of cylE on a plasmid vector.
17 ivo gene transfection approach using a naked plasmid vector.
18 egration-free human iPSCs from blood MNCs by plasmid vectors.
19 ovalent joining of DNA fragments to suitable plasmid vectors.
20 caused by multisite integration of viral or plasmid vectors.
21 ression system are contained in two separate plasmid vectors.
22 entially displayed bands were subcloned into plasmid vectors.
23 viral or bacterial recombinants, peptides or plasmid vectors.
24 of a cotransfected gene relative to standard plasmid vectors.
25 ach ORF were PCR amplified and inserted into plasmid vectors.
26 d EST-specific mRNA and cloned directly into plasmid vectors.
27 e or RNase L alone and leaves containing the plasmid vector alone produced typical systemic infection
28 ) and high (H) levels of expression, and the plasmid vector alone was transfected into M12 as a contr
31 d recombination in mammalian cells between a plasmid vector and a donor oligonucleotide was detected
32 tant improved expression from a conventional plasmid vector and from a Semliki Forest virus derived,
33 promoter region was cloned on an H. halobium plasmid vector and introduced into NRC-1 and S9, a bop o
34 excision of the transgene cassette from the plasmid vector and its permanent insertion into the geno
36 restriction fragments of genomic DNA into a plasmid vector and screened for recombinant plasmids con
37 re incorporated into a single-strand shuttle plasmid vector and used to establish the mutational freq
39 genome with a composite Ori but lacking the plasmid vector, and a molecule consisting of the remaini
40 upon complementation with the sof gene on a plasmid vector, and heterologous expression of sof49 in
41 Random mutations in porB were generated in a plasmid vector, and mutant gene pools were transformed i
43 oduct is similar to that from the retroviral plasmid vector, and the representation of different inse
44 of H. ducreyi were cloned independently into plasmid vectors, and their encoded proteins expressed si
45 een bla and lacZ on the standard lacZ fusion plasmid vectors; and (6) the single-copy construct flank
50 from 100 to 200 CAGs in a yeast integrating plasmid vector by taking advantage of replication instab
52 uorescent protein (GFP) from a microinjected plasmid vector can be suppressed in zebrafish embryos by
54 g a high-grade glioblastoma cell line with a plasmid vector capable of expressing an antisense transc
55 nipulation of C. diphtheriae, we constructed plasmid vectors capable of integrating into the chromoso
56 f green fluorescent protein (GFP) in which a plasmid vector carries a microsatellite repeat that plac
57 ransfected with empty plasmid vector or with plasmid vector carrying wild-type or mutant XRCC1 gene a
66 istent with mutational spectra observed when plasmid vectors containing dG-AAF or dG-AF are introduce
70 flhA in trans, an flhA mutant containing the plasmid vector control, or an fliC mutant (nonmotile mut
71 eatment with the IFN-alpha1 transgene or the plasmid vector control, with 0% survival following HSV-1
75 Expression of a recombinant F gene by use of plasmid vectors demonstrated that F contains its own tar
77 e by repressor titration, using the new pORT plasmid vectors designed to facilitate recombinant DNA e
79 y of the Cowden PEC genome was cloned into a plasmid vector directly downstream from the T7 RNA polym
81 ocardial injection of angiogenic peptides or plasmid vectors during open heart surgery in patients.
82 can be corrected, and indicate the value of plasmid vector encoding appropriate chemokines to achiev
84 ontrast to vectors encoding native beta-gal, plasmid vectors encoding beta-gal with a destabilizing r
85 der effect of the TRAIL gene, we constructed plasmid vectors encoding GFP-TRAIL or GFP-Bik chimeric p
87 y, the clpC gene cloned into a multiple-copy plasmid vector exhibited an activation phenotype, sugges
88 tion, cotransfection of HDV replicons with a plasmid vector expressing a hygromycin resistance marker
89 nescent dermal fibroblasts with a selectable plasmid vector expressing the SV40 T-antigen gene result
91 s that had been transiently transformed with plasmid vectors expressing E proteins that were mutant i
96 r by transfection of uninfected cells with a plasmid vector followed by infection with an F13L deleti
97 ine sequence was expressed from a eukaryotic plasmid vector following transfection into COS-1 cells.
100 ents (HRSE) was incorporated separately into plasmid vectors for generation of self-complementary ade
101 We report the development of a series of plasmid vectors for the construction of fusions to mutan
103 iously described to provide a large suite of plasmid vectors for use in this and other related Gram p
104 atest transformation efficiencies, while the plasmid vector had no significant effect, nor did the de
110 ia psittaci genomic library in a pBluescript plasmid vector in vitro, trapping EUO-bound plasmid clon
111 on in vitro and transferred into E. coli via plasmid vectors in the absence of the cognate methylase.
112 ave used EM visualization of active genes on plasmid vectors in Xenopus oocyte nuclei to investigate
114 in software for codon selection (CodonZ) and plasmid vectors incorporating the most active non-coding
116 nsduction of mecA from K1M200 (cloned into a plasmid vector) into a methicillin-susceptible S. aureus
117 uggest that systemic administration of naked plasmid vector is a convenient, safe, and highly efficie
118 red because when cloned on a low-copy-number plasmid vector it was able to suppress the temperature-s
122 ession of the protein in feline cells from a plasmid vector made them largely resistant to FPV infect
123 ts was hindered by CTG repeat instability in plasmid vectors maintained in Escherichia coli and poor
124 and precise transfer of DNA segments between plasmid vectors, makes this technology ideal for genomic
127 producing each E. coli protein from the 4287 plasmid vectors of the ASKA library and selecting for in
128 ells and EM-C11 cells transfected with empty plasmid vector or with plasmid vector carrying wild-type
129 was able to support replication in cis of a plasmid vector otherwise unable to replicate, if an inta
130 Co-expression of this plasmid with a second plasmid vector over-expressing the E. coli chaperonin pr
131 thelial cells were transfected in vitro with plasmid vector pcDNA:IGF-1, which encodes an epitope-tag
132 P-selectin, were cloned into a pUC19-derived plasmid vector, pCW93, and a pACYC184-derived phagemid v
133 re stably transfected with a hFIX expression plasmid vector, pdLMe4 betaA-hIXm1, which contains a hFI
134 xanthus phage Mx8 genome, when cloned into a plasmid vector, permits site-specific integration of the
141 yeast with the PCR fragment and a linearized plasmid vector prepared such that the ends of the vector
142 by expression of the URE gene in a mammalian plasmid vector (pSecTag2A.URE) which was used to immuniz
143 mid vector (pGEM11), one conventional binary plasmid vector (pSLJ1711) and one conventional binary co
144 njectable muscle-specific synthetic promoter plasmid vector (pSP-HV-GHRH), elicits growth in pigs.
146 n an antisense orientation in S. aureus on a plasmid vector reduces alpha-toxin production and the le
147 an intact copy of the S. iniae pgm gene on a plasmid vector restored antimicrobial peptide resistance
148 introduction of the nine-gene sag locus on a plasmid vector restored SLS activity to the nonhemolytic
149 nhibit TGF-beta expression with an antisense plasmid vector resulted in a significantly higher number
150 venous injection of human HGF gene via naked plasmid vector resulted in abundant HGF protein specific
151 eplication was an AAV genome inserted into a plasmid vector, RPA was not an effective substitute for
152 taining varying amounts of flanking gene and plasmid vector sequences were then introduced as linear
153 the bacterial neomycin-resistance gene in a plasmid vector, such that the reading frame of the neo g
156 2 glycoprotein D (gD), using combinations of plasmid vector that expresses gD (pgD2) and a recombinan
157 -KBP following transient transfection with a plasmid vector that expresses murine CD40, but not when
158 between 3 and 5 kbp in length on a multicopy plasmid vector that was transformed into E. coli to scre
162 oli cells transformed with any of the common plasmid vectors that provide ampicillin resistance throu
163 macrophages are difficult to transfect with plasmid vectors, these studies illustrate that primary m
164 flaviviruses, we have developed a eukaryotic plasmid vector to express the premembrane/membrane and e
166 roup (0/8) compared with levels expressed in plasmid vector-treated controls (4/6 mice surveyed were
167 d the infection to a greater extent than the plasmid vector-treated counterpart and at a level simila
168 ia virus type 1 (HTLV-1) was inserted into a plasmid vector under the control of the SP6 promoter.
170 disrupted is amplified by PCR, cloned into a plasmid vector using topoisomerase and then employed as
176 uberculosis DNA cloned upstream of inhA in a plasmid vector, was electroporated into M. tuberculosis,
183 in was sufficient for the replication of the plasmid vector when Rep and adenovirus (Ad) helper funct
185 were co-expressed in Escherichia coli on one plasmid vector with each cDNA having its own IPTG-induci
187 hnique to clone single oligonucleotides into plasmid vectors with high efficiency that predictably re
188 the loss frequencies of some low copy number plasmid vectors with parS inserts, as well as that of P1
189 sporting such hormones when overexpressed on plasmid vectors (with some demonstrable specificity obse
190 ontrols, mice were immunized with either the plasmid vector without an osp-coding sequence or recombi
191 ess high levels of immunogenic antigens from plasmid vectors without the need for antibiotic selectio
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