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1 lls because these surface structures are sub-light microscopic.
2                                              Light microscopic analyses have shown that both subunits
3                                              Light microscopic analyses of male meiosis in these plan
4                                     Previous light microscopic analyses of these mice left open quest
5                Double-immunofluorescence and light microscopic analyses revealed that both group I mG
6                                              Light microscopic analyses revealed that choline acetylt
7                                Unexpectedly, light microscopic analyses showed a dramatic loss of the
8                                              Light microscopic analyses showed that labeled axons rea
9        We present here detailed electron and light microscopic analyses that provide new insight into
10                                         Both light microscopic analysis and staining with the pan-neu
11                                              Light microscopic analysis demonstrated GLY-IR profiles
12                                              Light microscopic analysis demonstrated that erythrocyte
13                                              Light microscopic analysis in both Collins- and glycine-
14                                              Light microscopic analysis indicated that CRF processes
15                                              Light microscopic analysis of 11 biocytin-filled cells s
16                                              Light microscopic analysis of detached retinas showed th
17                                              Light microscopic analysis of ENK and GABA immunoreactiv
18                                              Light microscopic analysis of the optic nerve, chiasm, a
19                                              Light microscopic analysis revealed four populations of
20                                              Light microscopic analysis revealed oval or circular imm
21                                              Light microscopic analysis revealed prominent kappaOR im
22                                              Light microscopic analysis shows extensive glomerular di
23                                              Light microscopic analysis using Neurolucida tracings of
24  cells into mature fiber cells, as judged by light microscopic analysis.
25                Here, we describe FLASH (fast light-microscopic analysis of antibody-stained whole org
26                                              Light-microscopic analysis of semi-thin sections reveale
27      To overcome limitations of conventional light-microscopic analysis, we used high resolution Rama
28  colocalization in this material at both the light microscopic and electron microscopic levels sugges
29 ction compartment of these cells at both the light microscopic and electron microscopic levels.
30  and distorted NMJs were evident at both the light microscopic and electron microscopic levels.
31 m bovine molar teeth and studied at both the light microscopic and electron microscopic levels.
32 holaminergic neurons) and examined with both light microscopic and electron microscopic methods.
33      Animals were perfused and processed for light microscopic and electron microscopic study of both
34                               By integrating light microscopic and EM data, we estimate that sprouted
35 esting in GLT1 knock-out mice, were used for light microscopic and EM-ICC.
36 uts from two eyes, although there are subtle light microscopic and physiological differences.
37  of 8 months of age by routine techniques of light microscopic and scanning electron microscopy.
38                                              Light microscopic and ultrastructural analysis revealed
39 and perivascular mesenchymal cells appear by light microscopic and ultrastructural criteria to be fib
40 ichia coli (EPEC) on the basis of postmortem light microscopic and, in some cases, microbiological ex
41          In the present study, complimentary light microscopic anterograde biocytin and retrograde ho
42                                              Light microscopic anterograde tract-tracing studies have
43 We recently developed a multi-label confocal light microscopic approach that makes possible the syste
44                         We used electron and light microscopic approaches to unravel the roles of fib
45 g RNAi and is well suited to high-resolution light microscopic assays.
46                In accord with these results, light microscopic autoradiography of the rat brain showe
47 e evaluated with receptor binding assays and light microscopic autoradiography, using 1-2 nM [3H]pire
48                                        Using light microscopic autoradiography, we observe heavy labe
49  NTS had neither proteinuria nor significant light microscopic changes, yet had increased uptake of [
50 t appositions (18/21; 85.7%) selected by our light microscopic criteria were confirmed as direct cont
51 ns (3/21; 14.3%) selected as contacts by our light microscopic criteria were in fact separated from t
52  axon/myelin segmentation using a dataset of light-microscopic cross-sectional images of osmium tetro
53 t selected optical levels for correlation of light microscopic data and electron microscopic detail.
54                                        These light microscopic data suggested that neurons in the PGi
55                          Consistent with the light microscopic data, ultrastructural analysis showed
56                                 Quantitative light microscopic densitometry of the superficial dorsal
57                                 Quantitative light microscopic densitometry of the superficial dorsal
58  management of thyroid neoplasms is based on light microscopic diagnosis, but its accuracy and precis
59 vity was seen in processes having a regional light microscopic distribution comparable to that of kno
60               In this study, we describe the light microscopic distribution of CGRP immunoreactivity
61     Specificity also was demonstrated by the light microscopic distribution of KT-LI in sections thro
62    In the present report we have defined the light microscopic distribution of preganglionic negative
63 ghout the rat brain corresponds to the known light-microscopic distribution of VGLUT3.
64                                              Light microscopic double labeling immunocytochemistry fo
65                                              Light microscopic double-labeling immunoperoxidase exper
66                           A semiquantitative light microscopic evaluation of 1-mum-thick sections inc
67  staining were then compared to the standard light microscopic evaluation of the biopsies for rejecti
68 degree of deefferentation was quantified via light microscopic evaluation of the density of OCB fasci
69 ed before histopathology to allow for direct light microscopic evaluation of the lenses.
70                            Physiological and light microscopic evidence suggest that substance P (SP)
71                                  We produced light microscopic evidence that the axons of rostral VLM
72 upporting structures were processed for both light microscopic examination and immunohistochemical st
73                                              Light microscopic examination disclosed survival of the
74                                              Light microscopic examination of adult tissue revealed n
75                                              Light microscopic examination of an enucleated globe as
76                                              Light microscopic examination of brain, kidney, and sple
77                                     Based on light microscopic examination of Congo red-stained secti
78 re treated with Masson's trichrome stain for light microscopic examination of muscle fibers (red) and
79 urring inversions, identical at the level of light microscopic examination of polytene chromosomes, m
80                        In the present study, light microscopic examination of the immunohistochemical
81                                              Light microscopic examination of the mouse hippocampal f
82                                              Light microscopic examination of the PIMI and Linplant a
83                                              Light microscopic examination of the retinas showed that
84                                              Light microscopic examination revealed free blood island
85                                              Light microscopic examination revealed that DOX-induced
86                                   Polarizing light microscopic examination showed alternating light a
87                                              Light microscopic examination showed only loss of RGCs a
88                                            A light microscopic examination was performed to study the
89 airs of neurones could not be predicted from light microscopic examination.
90 owed widespread, microvesicular steatosis on light-microscopic examination, but only electron-microsc
91                         Gross pathologic and light microscopic examinations of each organ, as well as
92 MS, originally characterized on the basis of light microscopic features, are driven by fundamentally
93                                However, this light microscopic finding does not guarantee that NMDA r
94 ormed and the results were correlated to the light microscopic findings on traditional hemotoxyin and
95                                     IVCM and light microscopic findings suggest that the central corn
96                                              Light microscopic findings were recorded.
97 gions and dentate gyrus, and, in contrast to light microscopic findings, in nuclei of a few pyramidal
98                                     However, light microscopic histological analysis showed minimal h
99 ult without macular disease were compared to light microscopic histology from comparable ages.
100         Diagnosis is usually accomplished by light microscopic identification of spores in body fluid
101 ained or immunohistochemically stained whole light microscopic images (200 x) were acquired (15.61 TB
102 ll subset of podocytes enabled us to acquire light microscopic images of podocyte foot processes in u
103                                   High-speed light microscopic images of swimming T. primitia cells s
104                                              Light microscopic images were captured in 32 regions of
105 y of myelinated peripheral nerve fibers from light microscopic images.
106 non-fluorescence based phenotyping to enable light microscopic imaging modalities.
107 n be accomplished at low cost, and can allow light microscopic imaging of cleared tissues, thus enabl
108                                     By using light microscopic immunocytochemistry and computer analy
109                                        Using light microscopic immunocytochemistry and freeze-fractur
110                                      We used light microscopic immunocytochemistry and ultrastructura
111 as localized in normal human brain tissue by light microscopic immunocytochemistry by using highly sp
112 ned recording of wheel-running activity with light microscopic immunocytochemistry for vasoactive int
113                                              Light microscopic immunocytochemistry indicated that exp
114                                              Light microscopic immunocytochemistry revealed reaction
115                                              Light microscopic immunocytochemistry revealed that gran
116                                              Light microscopic immunocytochemistry reveals presenilin
117                                              Light microscopic immunocytochemistry showed that dying
118  were injected with neurobiotin and shown by light microscopic immunocytochemistry to be multipolar c
119 MF pathway LENK levels, we used quantitative light microscopic immunocytochemistry to evaluate LENK l
120 hybridization techniques in combination with light microscopic immunocytochemistry to show that the t
121                                              Light microscopic immunocytochemistry using affinity-pur
122 cortex of the rhesus macaque was examined by light microscopic immunocytochemistry using an antibody
123                                              Light microscopic immunocytochemistry using antibodies t
124 at caudate putamen, by using immunoblots and light microscopic immunocytochemistry.
125 ntrol and Huntington's disease (HD) cases by light microscopic immunocytochemistry.
126          Corneas were fixed and prepared for light microscopic, immunohistochemical, and electron mic
127                                Here, we used light microscopic immunohistochemistry and multilabel im
128                                              Light microscopic immunohistochemistry was performed on
129                                        Using light microscopic immunohistochemistry we find that the
130 ked immunosorbent assay and was localized by light-microscopic immunohistochemistry.
131                                              Light microscopic immunolocalization was performed with
132                                        Using light microscopic immunoperoxidase method, it was identi
133  presence did not seem to correlate with the light microscopic injury pattern represented by balloone
134  controlled, they are ideal for quantitative light microscopic investigation of dynamic processes in
135                                         This light microscopic investigation provides a detailed qual
136 f the alpha(1F) subunit were examined at the light microscopic level and by immunohistochemistry.
137 f this model, including visualization at the light microscopic level and direct analysis of virus pro
138 the frequency of VND was accomplished at the light microscopic level and validated by ultrastructural
139    Analysis of synaptotagmin labeling at the light microscopic level during development of the antenn
140     Retinal morphometry was performed at the light microscopic level in caspase-3 mutant mice from PN
141 ation of ERbeta-immunoreactivity (ir) at the light microscopic level in many brain regions and the id
142 mmunoreactive processes were apparent at the light microscopic level in the hypoglossal nucleus, but
143 phosphatase calcineurin was localized at the light microscopic level in the rat hindbrain and spinal
144                                       At the light microscopic level p75(NTR) immunoreactive elements
145 red hippocampal neurons and rat brain at the light microscopic level showed enrichment of GRIP in GAB
146 e from intracellular labeling studies at the light microscopic level suggests that a single cochlear
147 trated specific immunoreactivity (IR) at the light microscopic level throughout the brain, spinal cor
148           Immunostaining was employed at the light microscopic level to selectively label large myeli
149 t of the light neuropil staining seen at the light microscopic level was due to the staining of dendr
150 f most collateral branches correlates at the light microscopic level with dendrites.
151 ection, GluR1 appears as small puncta at the light microscopic level, and is found in dendritic spine
152                                       At the light microscopic level, autoradiography shows cell nucl
153                                       At the light microscopic level, both ENK and PNMT varicose proc
154                                       At the light microscopic level, dense M2 staining was seen in t
155                                       At the light microscopic level, immunolabeling was prominent in
156                                       At the light microscopic level, intense immunoreactivity was ap
157                                       At the light microscopic level, labeled fibers within the supra
158 letion did not affect lung morphology at the light microscopic level, nor did it affect the distribut
159                                       At the light microscopic level, retrogradely labeled cells were
160                                       At the light microscopic level, the anti-TH and anti-DA reveale
161                                       At the light microscopic level, the biotin reactivity appears i
162 ptive terms for liver precursor cells at the light microscopic level, the cells included in these des
163                                       At the light microscopic level, the density of vesicular glutam
164                                       At the light microscopic level, the distribution pattern and ce
165                                       At the light microscopic level, the nob retina appeared to have
166                                       At the light microscopic level, the NTS and inferior olive cont
167                                       At the light microscopic level, there appeared to be increased
168                                       At the light microscopic level, there was light to moderate lab
169 lar colocalization of NR2A/B with NR1 at the light microscopic level.
170 ed the pattern of mu-ORi at the bright-field light microscopic level.
171 s primarily due to limited resolution at the light microscopic level.
172 ot affect growth or tissue morphology at the light microscopic level.
173 e increased staining density observed at the light microscopic level.
174 not differ from the wild-type protein at the light microscopic level.
175 t terminals of any type could be detected at light microscopic level.
176 ological features of microglial cells at the light microscopic level.
177 rameter by which to assess plasticity at the light microscopic level.
178  (GFAP) to label astrocytes were used at the light microscopic level.
179 ne-sparse interneurons and astrocytes at the light microscopic level.
180 is interspersed thoroughly with CentC at the light microscopic level.
181 nd presumptive boutons invest the PPT at the light microscopic level; (2) at the ultrastructural leve
182 s of photodamaged versus healthy skin at the light microscopic level; comparison of cell shape and ap
183 ere was no evidence of histopathology at the light microscopic level; however, ultrastructural studie
184                                       At the light-microscopic level, both group I mGluRs are express
185 erular structure was normal at the gross and light microscopic levels.
186 unolocalization studies at the electron- and light-microscopic levels supported the conclusion that m
187 d RGS10 protein in rat and mouse brain using light microscopic (LM) and electron microscopic (EM) imm
188 t 15-360 min after injury, and processed for light microscopic (LM) and electron microscopic (EM) sin
189  the animals were perfused and processed for light microscopic (LM) and electron microscopic (EM) vis
190 y against the N-terminal of the 5-HTT at the light microscopic (LM) level indicates that the 5-HTT is
191 considerable expense and low throughput, and light microscopic (LM) methods, which provide molecular
192 een alga and tissues of the garden pea for a light microscopic localization of lipid A in these eukar
193    A finding of practical importance is that light microscopic measurements of boutons were diagnosti
194                                              Light microscopic measures revealed that a significant d
195 ration was not detected with general purpose light microscopic methods in previous studies using seve
196                                        Using light microscopic methods with immunohistochemistry, ele
197 at would not be detectable by using standard light microscopic methods.
198 NA fragmentation and the ultrastructural and light microscopic morphological features of MNs followin
199          In the present study we performed a light microscopic, morphometric analysis of identified O
200                                              Light microscopic observation of NMJs that showed synapt
201 copic, stereologic calculation confirmed the light microscopic observation.
202 quantitatively along the cochlear spiral via light-microscopic observation of cochlear wholemounts im
203                                              Light microscopic observations demonstrated morphologic
204                                              Light microscopic observations of the basilar papilla st
205                                              Light microscopic observations of the secretion process
206                                              Light microscopic observations revealed dense CaMK stain
207 ocytochemistry of rat brain sections shows a light microscopic pattern that is suggestive of reactivi
208                              The most common light microscopic patterns were diffuse (53%), focal (28
209                        Therefore, we applied light microscopic postembedding immunostaining and optic
210                                  However, in light microscopic preparations it was common to observe
211 ices, intracellularly labeled, processed for light microscopic reconstruction, and compared to GC lay
212 transmission electron microscopic images and light-microscopic reconstructions.
213 e morphology of these clefts, from the first light-microscopic report up to recent three-dimensional
214                                           At light microscopic resolution, M(2) immunoreactivity (-ir
215 energic fibers in the lesioned hemisphere at light microscopic resolution; at electron microscopic re
216                                          Our light microscopic results show that NOS I, as defined ma
217                                              Light microscopic retinal morphology was similar in Wt a
218                     Using high magnification light microscopic screening, both qualitative and quanti
219 nylated dextran amine were examined by using light microscopic serial reconstruction and electron mic
220 n hypothalamus were investigated by means of light microscopic single- and double-label immunocytoche
221                                              Light microscopic studies have shown that endomorphin-1
222                                              Light microscopic studies involving Kit tyrosine kinase
223                                              Light microscopic studies of BFT-treated monolayers reve
224                                 In addition, light microscopic studies of fluorescently tagged protei
225                                In aged cats, light microscopic studies revealed significant decrease
226                                 Our previous light microscopic studies suggested that extension of sy
227                                      Routine light microscopic studies were performed in a total of 7
228                     Consistent with previous light microscopic studies, alpha2AAR-I was found in peri
229   Opioid receptors have been demonstrated by light microscopic techniques in fine cutaneous nerves in
230                                        Using light microscopic techniques, including retinal whole-mo
231  this copolymerization is well-studied using light microscopic techniques, structural consequences of
232  removal corresponds to ECM as determined by light microscopic visualization of the stained protein.

 
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