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1 ulture systems (CS) (a bioreactor system and petri dishes).
2 imulation such as tapping on the side of the Petri dish.
3 ved at the points where the cell touches the Petri dish.
4 rpendicular to the cuts in the center of the petri dish.
5 as collected with paper points and plated in Petri dishes.
6 al to the cultures on commercial polystyrene Petri dishes.
7 macroculture systems such as well plates and Petri dishes.
8 dues formed in the lids of 38 mm polystyrene Petri dishes.
9 dices grown monoxenically on bicompartmental petri dishes.
10 agarose gels of various compositions cast in Petri dishes.
11 ds in different ratios and placing them in a Petri dish after which they are recorded using a camera
13 ications of SM imaging techniques beyond the petri dish and opens the possibility to explore the mole
15 membrane (CAM) of quail embryos cultured in petri dishes and incubated for an additional 24 or 48 ho
17 lar bag was dissected free, pinned flat on a petri dish, and incubated in Eagle's minimal essential m
18 chemokines are applied onto the surface of a Petri dish, and then immersed under culture medium in wh
19 ng cocultivation with seedlings in bipartite Petri dishes, and (35)S was assimilated from the bacteri
22 ental setup suggested uses opaque masks in a Petri dish bathed in ultraviolet radiation, but is based
23 into one macroscopic fluorescent plaque in a Petri dish by plating it in a host bacterial medium.
24 ies grown on glass slides and in polystyrene petri dishes by using light microscopy and scanning and
25 aining two compartments (BI Petri dish); two Petri dishes connected with tubing; and a microtiter-bas
26 r Arabidopsis or tobacco plant seedlings): a Petri dish containing two compartments (BI Petri dish);
27 were removed and were replaced with sterile petri dishes containing a droplet of sterile brucella br
28 netic field attraction (deflection angle and Petri-dish displacement methods), heating (infrared ther
30 les, in a lawn of bacteria on an agar-filled Petri dish; however, this rate-limiting step requires up
32 patially extended bacterial populations in a Petri dish is presented on the basis of an exact formula
33 ecombinant protein to type I collagen-coated Petri dishes is inhibited by anti-65m in a dose-dependen
34 e substrates including polydimethylsiloxane, Petri dishes, Kapton tapes, thermal release tapes, and m
35 in neither binds to type III collagen-coated Petri dishes nor inhibits type III collagen and ADP-indu
37 0 droplets/mm2) sprayed on the bottom of the Petri dish, or by flushing N2 above the heptane, the mic
38 ansferred into standard 96-/384-well plates, Petri dishes, or vials for cloning, PCR, and other singl
39 t this technology can be used to build smart Petri dish platforms, termed ePetri, for cell culture ex
44 ide FOV time-lapse fluorescence self-imaging Petri dish system, termed the Talbot Fluorescence ePetri
45 e are printed in seconds on plastic or glass Petri dishes; then, interfacial forces pin liquids to su
47 a Petri dish containing two compartments (BI Petri dish); two Petri dishes connected with tubing; and
49 sected alimentary tracts, and excreta on the petri dishes were cultured for H. pylori, whose identity
51 iological and histological analysis, and the petri dishes were replaced with fresh sterile plates wit
53 for cell immobilization included coating the Petri dish with 100 microg/mL fibronectin, a seeding cel
54 living bacterial colonies directly from the Petri dish with absolutely no sample preparation needed.
55 atory diagnosis could be made using only one petri dish with sliced agar, thereby saving time and med
56 ion of human neutrophils adherent to plastic petri dishes with the purified chemotactic factors C5a a
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