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1 ontal pockets with PD of >/=5.4 mm, a single subgingival administration of a 0.4% moxifloxacin gel as
2 is study was to compare trehalose powder for subgingival air-polishing with sonic debridement in resi
6 s were randomly assigned to receive a single subgingival application of a 0.125%, 0.4%, or 1.25% moxi
7 tive periodontal pathogens and resistance of subgingival bacteria against moxifloxacin were assessed.
8 ined potential correlations between detached subgingival bacteria collected in gingival crevicular fl
9 obial mouthrinse on levels of representative subgingival bacteria in subjects with mild to moderate p
10 ion on the prevalence and levels of selected subgingival bacteria using molecular approaches for bact
12 of local inflammation on the composition of subgingival bacteria, and 3) to understand how inflammat
13 determine the effect on clinical variables, subgingival bacteria, and local immune response brought
14 mographics, PD, clinical loss of attachment, subgingival bacteria, serum hsCRP, interleukin (IL)-1bet
16 , a chronic inflammation driven by dysbiotic subgingival bacterial flora, is linked on clinical level
19 ts did not sterilize or substantially reduce subgingival bacterial populations compared to negative c
20 study characterizes the association between subgingival bacterial profile and periodontal parameters
23 ngival crevicular fluid (GCF) biomarkers and subgingival bacterial species in periodontally healthy s
26 l role for smoking cessation in altering the subgingival biofilm and suggest a mechanism for improved
27 effects on major periodontopathogens in the subgingival biofilm as well as on biomarkers in the ging
28 that SubGPAP is more efficacious in removing subgingival biofilm in moderate-to-deep periodontal pock
31 Aggregatibacter actinomycetemcomitans in the subgingival biofilm of individuals with and without seve
32 hing appears to be a promising procedure for subgingival biofilm removal in periodontal treatment.
34 studies comparing microbiologic outcomes of subgingival biofilm samples from healthy implants and im
39 is is related to the presence of a dysbiotic subgingival biofilm that elicits the immune response.
42 sythia (previously T. forsythensis) in their subgingival biofilm was determined by polymerase chain r
43 forsythia, and Fusobacterium nucleatum from subgingival biofilm were determined by quantitative poly
45 olymerase chain reaction on the basis of the subgingival biofilm, and IL-1beta and TNF-alpha were qua
46 of periodontitis; however, its effect on the subgingival biofilm, the primary etiological agent of pe
47 ts the composition of the disease-associated subgingival biofilm, yet little is known about its effec
51 d by significant changes in the marginal and subgingival biofilms, with a decrease in the abundance o
52 le initial colonization of both marginal and subgingival biofilms, with lower niche saturation than t
55 levels, bleeding upon probing, or extent of subgingival calculus comparing subjects assigned to prot
56 the 655-nm InGaAsP diode laser in detecting subgingival calculus in patients with periodontal diseas
57 associations between bone density, CAL, and subgingival calculus require further research, particula
58 ulus deposition over tooth surfaces, and the subgingival calculus that enables the enlargement of the
59 ratively a mucoperiostal flap was performed, subgingival calculus was visualized, and photographic im
60 The overall probability to correctly detect subgingival calculus with the laser (accuracy) was 0.82
61 ans with type 2 diabetes had more supra- and subgingival calculus, an increased extent and severity o
67 ures on restoration of microbial eubiosis in subgingival communities, confirming the important role f
68 ed to perform a directed survey of the human subgingival crevice and to isolate bacteria having rod-l
70 ts were identified who underwent surgery for subgingival curettage and/or periodontal flap and are co
71 riodontal disease who undergo procedures for subgingival curettage and/or periodontal flap have a rem
73 group (one session of full-mouth ultrasonic subgingival debridement followed 1 week later by Er:YAG
74 ip (CHX chips) as an adjunctive treatment to subgingival debridement in patients afflicted with peri-
75 (Er:YAG) laser application as an adjunct to subgingival debridement in the treatment of chronic peri
77 ssesses the efficacy of combining full-mouth subgingival debridement with Er:YAG laser application in
78 ed (SLA) titanium disks were inoculated with subgingival dental plaque and cultured anaerobically for
79 onstellatus and Streptococcus intermedius in subgingival dental plaque biofilms may contribute to for
81 g the restorative phase of treatment, and in subgingival dental plaque of periodontitis patients, ind
82 cter rectus, and Fusobacterium nucleatum, in subgingival dental plaque of pregnant women in the OPT S
85 al flap surgery is frequently used to remove subgingival deposits, yielding consequential reductions
86 gh-throughput in vitro model that replicates subgingival dysbiosis and normobiosis, with a tool to me
89 evealed poor in vitro activity against human subgingival E. faecalis clinical isolates, and would lik
90 developed to facilitate visualization of the subgingival environment as an aid in diagnosis and non-s
94 lant pocket depths (IPD) of 5-8 mm underwent subgingival implant surface debridement followed by repe
96 eatment outcome after 12 months of different subgingival irrigation solutions during scaling and root
97 is known of the antibiotic susceptibility of subgingival isolates of these two bacterial species, thi
102 -mouth clinical measures of extent/severity, subgingival microbial burden by several species, and sel
103 eractions between the host immune system and subgingival microbial communities during the resolution
105 ing cessation altered the composition of the subgingival microbial community, by means of a quantitat
106 e next-generation sequencing to evaluate the subgingival microbial composition of young patients with
107 ompiled the results of all studies comparing subgingival microbial data between these clinical condit
108 reports, case series, and reviews) comparing subgingival microbial data from patients with CP and AgP
109 monstrated that smoking cessation alters the subgingival microbial profile; however, the response of
110 ailable data on clinical periodontal status, subgingival microbial profiles, and serum IgG antibodies
111 ng (BOP), plaque index (PI), and count of 40 subgingival microbial species (checkerboard DNA-DNA hybr
112 Among older women, taxonomic differences in subgingival microbiome composition and diversity were ob
115 riodontal therapy and smoking cessation, the subgingival microbiome is recolonized by a greater numbe
116 sively assessed the changes occurring in the subgingival microbiome of young patients with periodonti
118 EMD treatment predictably alters a dysbiotic subgingival microbiome, decreasing pathogen richness and
123 to grow health- and periodontitis-associated subgingival microbiomes in parallel, and we describe a n
125 ncing was used to compare the composition of subgingival microbiota and establish correlations betwee
126 tudy was to quantify the association between subgingival microbiota and periodontal disease progressi
127 hese prospective results affirm clearly that subgingival microbiota are measurably elevated several y
129 gates HGF expression and its relationship to subgingival microbiota in medically healthy individuals
133 ective of this study was to characterize the subgingival microbiota of African-American children with
137 e and number of periodontal pathogens in the subgingival microbiota of smokers versus never-smokers w
138 t literature regarding the complexity of the subgingival microbiota of the domestic cat and reveal bo
139 t in patients with a metronidazole-sensitive subgingival microbiota on the clinical parameters of CAL
141 We investigated whether baseline measures of subgingival microbiota predicted fasting plasma glucose
143 translocation of periodontal pathogens from subgingival microbiota to the bloodstream and then to at
145 major differences in the composition of the subgingival microbiota were observed between shallow and
147 AgP periodontitis present differences in the subgingival microbiota when compared with patients with
148 he relationships among these biomarkers, the subgingival microbiota, and the clinical parameters of p
151 in health at low levels, but changes to the subgingival nutritional environment increase their compe
152 C. albicans) were more often present in the subgingival OB of patients with and without type 2 diabe
153 was to assess the presence of yeasts in the subgingival OB of patients with type 2 diabetes and peri
155 e investigated the presence of yeasts in the subgingival oral biofilm (OB) of type-2 diabetic and non
157 antimicrobial sensitivity of enterococci of subgingival origin, this study evaluates the in vitro an
162 fect of alcohol consumption on the levels of subgingival periodontal pathogens and proinflammatory cy
163 n vitro antibiotic resistance among selected subgingival periodontal pathogens in patients with CP.
164 h CP in the United States frequently yielded subgingival periodontal pathogens resistant in vitro to
165 rall, 74.2% of the patients with CP revealed subgingival periodontal pathogens resistant to at least
168 y failed to observe any adjunctive effect of subgingival placement of chlorhexidine chips after scali
169 clinical examination during which samples of subgingival plaque and buccal epithelial cells were obta
174 mean +/- SD, 34 +/- 10 y) from whom baseline subgingival plaque and longitudinal FPG were measured.
175 ed at baseline and after 3 and 6 months, and subgingival plaque and sulcus fluid samples were taken f
176 g of the bacterial species present in canine subgingival plaque and their associations with health an
178 hod to detect three periodontal pathogens in subgingival plaque collected before treatment and at 2 a
179 ipid extracts derived from diseased teeth or subgingival plaque do not contain free lipid A constitue
183 laser on titanium surfaces contaminated with subgingival plaque from patients with peri-implantitis a
185 [MMP]-8, elastase, and sialidase) in GCF and subgingival plaque levels of Porphyromonas gingivalis, T
187 Changes in individual species levels in subgingival plaque microbiota were not detectable; howev
188 strain D11S-1, which was recovered from the subgingival plaque of a patient diagnosed with generaliz
189 ntal examination was performed, and a pooled subgingival plaque sample was collected from the deepest
195 ase chain reaction analysis was performed on subgingival plaque samples for the detection of A. actin
198 of different bacterial species in saliva and subgingival plaque samples from individuals with aggress
199 ecies biofilms were derived using supra- and subgingival plaque samples from mesio-buccal aspects of
207 nt positive correlation between salivary and subgingival plaque samples was detected in patients with
219 n to clinical measurements and GCF sampling, subgingival plaque samples were collected from four post
239 t be discussed as a potential alternative to subgingival plaque sampling for microbiologic analysis i
245 probing, and plaque index were measured, and subgingival plaque was collected from LAgP diseased and
250 regatibacter actinomycetemcomitans levels in subgingival plaque were analyzed by quantitative real-ti
251 aseline, gingival crevicular fluid (GCF) and subgingival plaque were collected and clinical periodont
254 all the samples (saliva, supragingival, and subgingival plaque) and was correlated with AAA diameter
256 s included a periodontal examination; blood, subgingival plaque, and crevicular fluid specimen collec
258 dontitis, is abundant at the leading edge of subgingival plaque, where it interacts with gingival epi
259 ion to the highly proteolytic environment of subgingival plaque, which is exposed continually to an a
268 ence of all three species in the reservoirs (subgingival pockets and blood DCs) of PD patients before
269 in reducing clinical parameters of LAgP and subgingival presence of JP2 in diseased and healthy site
275 gnosed with severe chronic periodontitis had subgingival samples harvested from four sites (the deepe
279 tal, 44 domestic cats were enrolled, and 139 subgingival samples were subjected to 16S rRNA gene sequ
280 T. forsythia, or C. rectus) were detected in subgingival samples, with a prevalence rate of 72.2%, 47
285 temic antibiotics or with plaque control and subgingival scaling significantly reduces CRP levels aft
286 ent and CMV was rarely present in individual subgingival sites affected by chronic periodontitis.
287 surfaces-is also a significant colonizer of subgingival sites in patients with chronic periodontitis
288 rease in microbial diversity was observed in subgingival sites of ailing implants, compared with heal
290 to periodontal breakdown in heavily infected subgingival sites, particularly in patients responding p
293 aim of the present study is to analyze which subgingival species are associated with SUP in patients
294 of 33 S. constellatus and 17 S. intermedius subgingival strains, each recovered from separate patien
295 was developed to aid in the visualization of subgingival structures and to improve the diagnosis and
296 al crevicular fluid (GCF) and a selection of subgingival/submucosal plaque bacteria from clinically h