MICROBIOLOGY OF THE DENTAL IMPLANT T

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MICROBIOLOGYOF THE DENTAL IMPLANTA . MOMBELLIUniversity of BernSchool of Dental MedicineFreiburgstrasse 7CH-3010 Bern, SwitzerlandAdv Dent Res 7(2):202-206, August, 1993Abstract—Longitudinal studies have shown that successfulimplants are colonized by a predominantly Gram-positive,facultative flora, which is established shortly after implantation.Repeated microbiological sampling in patients with clinicallystable implants showed no significant shifts in the compositionof this flora over five years. In patients with bone loss andpocket formation around implants, however, a significantlydifferent flora was found: Gram-negative anaerobic bacteria,particularly fusobacteria, spirochetes, and black-pigmentingorganisms such as Prevotella intermedia were often present inhigh proportions. Antimicrobial treatment with agentsspecifically active against anaerobes could halt progression ofperi-implant infections in such cases. Although there may benon-microbial primary causes for implant failure, these studiesshow that Gram-negative anaerobes may play a role in periimplant infections, and that their elimination leads toimprovement of the clinical condition.Terms such as "failing implant", "early" and "late failure",and "peri-implantitis" have been proposed forpathological states of osseointegrated implants and theirsurrounding tissues. There is no terminology which hasgenerally been agreed upon: Definitions and etiologies of theseconditions are still a matter of dispute. Essential information onthe biology of peri-implant tissues is still lacking. Diagnosis andtreatment of the different conditions are based primarily onmechanical contemplations; force distributions, load andphysical stress, properties of materials, implant design, themacroscopic arrangement and appearance of tissues, andsurgical skills are the traditionally considered factors. There isno doubt that mechanical problems, e.g., the fracture of animplant, can give rise to biological problems such as a secondarybacterial infection in the peri-implant tissues. However, there isalso the possibility that bacterial factors initiate tissue changeswithout an underlying mechanical cause.Tissue integration depends on eukaryotic cell compatibilityand adhesion to the implant surface. Fundamental physical andmolecular principles of cell attachment and adhesion apply tomicrobial colonization and host-tissue integration (Gristina,1987). Thus, it is conceivable that implant materials, which arechosen because of their "friendliness" to tissue cells, offerparticularly favorable grounds for bacterial adhesion. Pocketformation and loss of bone in the peri-implant area indicatedetachment of host tissue cells and availability of "cell-friendly "surfaces for microbial colonization. Adhesion-mediatedinfections developing on permanently or temporarily implantedbiomaterials, such as heart valves, vascular prostheses, orintravascular catheters, respond poorly to antimicrobialtreatment and often require that the device be removed. Dentalimplants, however, can be designed in such a way that thesurfaces on which bacterial colonization occurs may be reachedfrom the exterior. Thus, in contrast to internal implants, thereis a possibility for control of bacterial colonization on exposedsurfaces and a potential for treatment of infectious conditionsof peri-implant tissues.INITIAL COLONIZATION ANDBACTERIOLOGY OF STABLE IMPLANTSPresented at the 12th International Conference on OralBiology (ICOB), "Modern Concepts in the Diagnosis ofOral Disease", held at Heriot-Watt University, Edinburgh,Scotland, July 6-7,1992, sponsored by the InternationalAssociation for Dental Research and supported by UnileverDental Research202Microbial adhesion and aggregation have been studied ondifferent substrata, in vivo and in vitro (for review, seeMergenhagen and Rosan, 1985). Few publications, however,have addressed the interactions between bacteria and oralimplant materials such as titanium (Nakazato et a/., 1986;Fujioka-Hirai et al.9 1987; Joshi and Eley, 1988; Wolinsky etal., 1989). Likewise, general growth and maturation patternsof bacterial plaque have been studied by light and electronmicroscopy and bacterial culture (for review, see Theilade andTheilade, 1985), but, so far, only two investigations havefocused on the development of plaque on newly insertedimplants (Nakou et al., 1987; Mombelli et ai, 1988). In

VOL.7(2)MICROBIOLOGY AND IMPLANTSedentulous patients, the flora developing on successfullyintegrating one-stage transmucosal titanium implants was foundto be very similar to the mucosal flora on the adjacent alveolarridge (Mombelli et al, 1988). This flora was establishedshortly after the installation of the implant. Over 85% of themicro-organisms were identified, in the microscope, as coccoidcells, and over 80% of the cultivated bacteria were Grampositive facultative cocci. During the first six months afterinsertion, no significant longitudinal changes were noted inthese proportions. Spirochetes were never detected;Fusobacteria and black-pigmenting Gram-negative anaerobeswere found infrequently. The microflora associated with stableosseointegrated implants serving successfully as abutmentsfor overdentures was investigated in 18 edentulous patients,two years after implantation (Mombelli and Mericske-Stern,1990). Over 50% of the organisms cultured in this study werefacultatively anaerobic cocci, and 17% were facultativelyanaerobic rods, while Gram-negative anaerobic rods accountedfor only 7%. Fusobacterium sp. and Prevotella intermediawere both found in 9% of the samples. Porphyromonasgingivalis and spirochetes were not found. Repeatedmicrobiological and clinical data were collected in nine patientsduring the third, the fourth, and the fifth years after implantation.No significant time trends were noted. Separate samples takenwithin the same patient from different sites showed a similarcomposition of the microflora. The data of this study are inagreement with results reported by Lekholm et al. (1986),Apse et al. (1989), and Bower et al. (1989) from successfulBranemark-type implants. This indicates that the normalmicrobial flora of ITI and of Branemark fixtures are notsubstantially different from each other. Intra-individualtopographical variation of the bacterial flora seems to be morepronounced in partially edentulous patients than in edentates.The microbiota of remaining teeth is probably the primarysource of putative pathogens to colonize adjacent implants.Apse et al. (1989) found higher percentages of black-pigmentingGram-negative anaerobes and "wet spreaders"(Capnocytophaga) on implants of partially edentulous patientsthan in edentulous patients. This means that the microbialstatus of remaining teeth influences the fate of newlyincorporated implants.BACTERIOLOGY OF THE FAILING IMPLANTThe first data on the microbiota associated with unsuccessfulimplants were presented by Rams and co-workers (Rams andLink, 1983; Rams et al, 1984). These investigators collectedsamples from 17 implants of various designs (ramus frameassembly, blade implants, carbon and ceramic posts) andanalyzed them by phase-contrast and in part by transmissionelectron microscopy. Among these implants were four failuresshowing advanced pocket formation. While the samples fromthe successful implants yielded a predominantly coccoidmicrobiota, the failures showed significantly elevated levels ofspirochetes.In 1987, we reported data from seven cases with unsuccessfulhollow cylinder titanium implants (ITI Type F). Implant siteswith pocket formation 6 mm, suppuration, and radiographicevidence for bone loss were compared with implant sites with203no signs of infection in the same individuals and in patientswith only successful implants (Mombelli et al., 1987). In theunsuccessful sites, a substantially different distribution ofbacterial morphotypes was found in comparison with healthysites in both the same patients and in the successful patients.While spirochetes were not found in any of the successful casesand in only two samples of the healthy sites of the unsuccessfulpatients, all but one failing site in these patients harboredspirochetes. Failing sites harbored significantly elevatednumbers of motile rods and fusiform bacteria. The total countof colony-forming units, determined by anaerobic culture, wassignificantly higher in the failing sites than in the healthy sites.In the samples of the failing sites, 41% of the cultivatedorganisms were Gram-negative anaerobic rods. This numberwas significantly higher than that of the successful sites, wherethe group of facultative cocci predominated. Failing sitesharbored significantly elevated numbers of P. intermedia andFusobacterium sp. P.gingivalis was not found in any of thesamples investigated in this study, neither culturally nor byindirect immunofluorescence.In the earlier-mentioned prospective study on themicrobiology of newly inserted implants (Mombelli et al,1988), the development of a peri-implant infection could bedocumented clinically and microbiologically in one patient.Clinical signs of infection, including pocket development andpus formation, emerged 120 days after implantation. Samplestaken before day 120 repeatedly yielded 106 CFU/mL ofanaerobically cultivable bacteria. Fusobacterium was detected42 days after implantation, with increasing numbers in thesubsequent samples. In this particular site, from day 21 on, asteady decrease of coccoid cells and a simultaneous increase ofrods were observed. Actinomyces odontolyticus was firstdetected after day 21, and fusobacteria were detected after day42; at day 120, small spirochetes were found for the first time,pus formation was noted clinically, and a pocket probing depthof 6 mm was recorded. None of the other sites showed pusformation or pocket depths of over 3 mm.These studies suggested that what was chosen to be called"peri-implantitis" was a site-specific disease process withmicro-organisms associated in patterns known from chronicperiodontitis of natural teeth. More recent studies haveconfirmed and extended these earlier findings. Sanz et al(1990) made comparisons between healthy and diseased andbetween implant and control sites in patients wearing endostealsapphire ceramic implants. Diseased sites harbored a microbiotawith a large segment of Gram-negative anaerobic rods, includingblack-pigmented organisms and surface translocators. Healthysites in the same patients yielded small amounts of bacteriawhich were mainly facultative and Gram-positive. Becker etal. (1990) used commercially available DNA probes to test forthe presence of the three periodontal marker organisms—Actinobacillus actinomycetemcomitans, P. intermedia, and P.gingivalis—in 36 failing implant sites of 13 patients withdifferent types of implants (blade-type, subperiosteal, androot-form-type). They reported high levels of P. gingivalis inone patient with a failing blade implant and high levels of P.intermedia in two additional patients with unsuccessful blades.In the other cases, some weak signals were obtained for one or

204ADV DENT RES AUGUSTMOMBELLIseveral of the three tested organisms. Alcoforado et al. (1991)examined the subgingival microflora of 18 failingosseointegrated implants of various designs (Br&nemark, CoreVent, Integral, Screw-Vent, and TPS) for potentially pathogenicoral bacteria. Peptostreptococcus micros was recovered from6 failing implants, Wolinella recta from 6, Fusobacterium sp.from 5, and P. intermedia from 4. The authors reportedsignificant numbers of enteric rods or pseudomonads in themicroflora of 5 failing implants. A. actinomycetemcomitans,non-pigmented Bacteroides species, Capnocytophaga sp., andstaphylococci were also detected in some implant failures. Inaddition, 5 cases were positive for Candida albicans. Based onthese findings, the authors suggested that antimicrobial therapiesfor implant failures should not be implemented without a priorcomprehensive microbiological analysis. Rams et al. (1990)also suggested that some peri-implant lesions may be dominatedby a specific microbiota. A limited number of their patientsdemonstrated particularly high counts of Staphylococcus sp.,implying that these organisms are possible pathogens undercertain conditions. Rosenberg et al. (1991) comparedmicrobiological features of implants suspected of failing frominfection or trauma. An infectious etiology was assumed ifthere was bleeding, suppuration, pain, high plaque and gingivalindices, and granulomatous tissue upon surgical removal.Implants were suspected of failing because of traumatic reasonsin the absence of these signs. Distinct bacteriologic profilesemerged in the two groups: Implants suspected of failingbecause of trauma demonstrated microbiological featuressimilar to those of periodontally healthy teeth, while manysuspected periodontal pathogens were found if clinical signssuggested infection.The role of micro-organisms in the development of periimplant pathology has also been investigated in animals.Differences in the presence of putative periodontal pathogenson titanium implants and teeth were determined in beagle dogsin experimental gingivitis and in a ligature-induced periimplantitis/periodontitis situation (Leonhardt et al., 1992).Similar colonization patterns were seen on implants and teeth.Significant microbiological differences between implants andteeth were found neither with gingivitis nor in ligature-inducedperi-implantitis/periodontitis.To summarize the data available today: There appears tobe a very clear microbiological distinction between clinicallystable implants and implants with peri-implant pathology.Undoubtedly, Gram-negative anaerobic bacteria are involvedin pathological developments in the peri-implant region.These organisms are also suspected pathogens in periodontitisand orofacial infections (for review, see Crawford, 1984;Van Steenbergen et al, 1991). Spirochetes can be perceivedas indicators for a flora with anaerobic characteristics. Theyare evidently not a feature of the physiological flora ofsuccessful implants.TREATMENT OF PERI-IMPLANTINFECTIONSSince anaerobic bacteria are associated with peri-implantpathology, the question arises of whether clinical conditionscan be improved by suppression or elimination of these1993organisms from affected sites. An antimicrobial therapeuticapproach was tested in a study involving nine patients withmarked loss of bone and pocket probing depths 5 mm aroundimplants (Mombelli and Lang, 1992). These patients wereselected based on microbiological screening; only individualswith anaerobic cultivable counts 106 CFU/mL, including 20% Gram-negative anaerobic bacteria, in diseased sites, wereconsidered. The treatment included mechanical debridement,irrigation of all peri-implant pockets 3 mm with 0.5%chlorhexidine, and systemic antimicrobial therapy with anagent specifically effective against strict anaerobes (ornidazole,1000 mg for ten consecutive days). After therapy, bleedingscores decreased immediately. Over a one-year observationperiod, they remained significantly lower than before treatment.A significant gradual reduction in mean probing depths wasdetected over this one-year period. Only one case showed noimprovement of local probing depth. Microbiologicalparameters indicated an instantaneous quantitative andqualitative change following treatment. Subsequently, severalof these parameters tended to shift back toward pre-treatmentvalues. In the second half of the observation period, however,this tendency was reversed, and levels significantly differentfrom baseline were eventually established. Most affected sitesharbored large numbers of Fusobacterium, and many were P.intermedia-positive before treatment. Although these organismscould no longer be detected upon completion of therapy, allpatients showed Fusobacterium again at some time during thefollowing year, and only three individuals remained P.intermedia-negativethroughout this period. Similarobservations could be made with the other organisms underinvestigation. Since no organism was consistently presentbefore and uniformly absent after therapy, the clinical successof the treatment cannot be attributed to the elimination of asingle pathogen. Rather, it seems that a temporary relief froma massive anaerobic bacterial load allowed local host-responsemechanisms to recover so that they could cope with reemerging opportunistic pathogens. While the immediate effectsof chemotherapy may fade away with time, gradual reductionin pocket depth, leading to a rise in oxygen partial pressure(pO2) and redox potential (Eh) (Loesche et al, 1983), togetherwith a reduced availability of blood products, may exert a longterm ecological pressure to stabilize a less pathogenicsubgingival microbiota. Because of the possibility that microorganisms other than strict anaerobes may be involved in somecases of peri-implant pathology (Rams etal, 1990; Alcoforadoet al., 1991), the choice of an antimicrobial drug should bebased on a comprehensive microbiological analysis.RECALLFrom periodontal research, it is known that the developmentof a complex microbiota with a large segment of Gramnegative, anaerobic bacteria depends on specific environmentalconditions, which are provided in part by facultative initialcolonizers (Van Houte, 1982; Socransky et al, 1988; TerSteeg and Van der Hoeven, 1990). It is also known that thedevelopment of a flora with a large proportion of Gramnegative anaerobes can be prevented by oral hygiene (Kornman,1982; Wolff et al, 1988). Flemmig et al (1989) reported

VOL.7(2)MICROBIOLOGY AND IMPLANTSabout the possibility of maintenance of an implant-associatedmicroflora without substantial proportions of suspectedperiodontal pathogens by recalling patients at three-monthintervals. Clinical and microbiological features of Branemarkimplants submitted to three-month recalls on a long-termbasis (Ericsson et al., 1986; Lekholm et al., 1986) seem toconfirm that this form of maintenance is effective. However,it cannot be excluded that three-month intervals meanovertreatment in many cases. In our longitudinal study on themicroflora associated with stable osseointegrated implantsin edentates (Mombelli and Mericske-Stern, 1990), the datacollected up to five years after implantation were analyzedfor evaluation of shifts in the composition of the microfloraover time and the impact of re-call intervals and selectedclinical parameters on microbiological features. In this study,patients on longer re-call intervals showed no significantdifference in the composition of the microflora, when comparedwith patients on short re-call intervals. Significant interindividual differences were found for proportions of P.melaninogenica and A. odontolyticus. This means that someindividuals were less susceptible to colonization and growthof certain dental plaque micro-organisms than others. Nogeneral time trends were observed during the longitudinalmonitoring phase in this study. Thus, the microbiologicalsituation could be maintained fairly stable after a successfullycompleted initial healing phase.CONCLUDING REMARKSA review of the research performed so far leads to the conclusionthat micro-organisms are involved in peri-implant pathology.There is evidence for an association of certain plaqueconstituents with tissue breakdown around implants.Antimicrobial treatment aimed at the reduction of anaerobicbacteria leads to improvement of clinical parameters.Nevertheless, it is premature to claim proof for a direct causeeffect relationship between specific pathogens and tissuedestruction. It has been repeatedly emphasized that numerousfactors may influence the health conditions of peri-implanttissues, particularly in the initial healing phase. Bacterialinfection may occur as a secondary phenomenon ifosseointegration is not achieved or is lost due to non-microbialreasons. It has been speculated that distinct types of failure maybe differentiated based on the presence or absence of the"typical" peri-implantitis flora (Rosenberg et al., 1991), andthat in some patients, specific infections may be the reason forimplant failure (Rams etal, 1990). These possibilities illustratethat microbiological tests may be valuable tools for thedifferential diagnosis of problems occurring withosseointegrated implants. Longitudinal, prospective studiesare needed for determination of whether microbiologicalparameters can indicate a risk of peri-implant tissue destructionor allow early disease states to be detected.REFERENCESAlcoforado GAP, Rams TE, Feik D, Slots J (1991). Aspectsbacteriologiques des echecs des implants dentairesosteointegres chez l'homme. Parodontologie 10:11-18.Apse P, Ellen RP, Overall CM, Zarb GA (1989). Microbiota205and crevicular fluid collagenase activity in theosseointegrated dental implant sulcus: A comparison ofsites in edentulous and partially edentulous patients. JPeriodontRes 24:96-105.Becker W, Becker BE, Newman MG, Nyman S (1990). Clinicaland microbiologic findings that may contribute to dentalimplant failure. Int J Oral Maxillofac Surg 5:31-38.Bower RC, Radny NR, Wall CD, Henry PJ (1989). Clinical andmicroscopic findings in edentulous patients 3 years afterincorporation of osseointegrated implant-supportedbridgework. / Clin Periodontol 16:580-587.Crawford JJ (1984). Orofacial infections and antibioticmanagement. In: Newman MG, Goodman AD, editors.Guide to antibiotic use in dental practice. Chicago:Quintessence, 25-38.Ericsson I, Lekholm U, Branemark P-I, Lindhe J, Glantz P-O,Nyman S (1986). A clinical evaluation of fixed-bridgerestorations supported by the combination of teeth andosseointegrated titanium implants. / Clin Periodontol13:307-312.Flemmig TF, Berwick RHF, Newman MG, Kenney EB, BeumerJ, Nachnani S, et al. (1989). Effekt des Recalls auf diesubgingivale Mikroflora von osseointegrierten Implantaten.Hamburg: Tagung des Arbeitskreises ftir Implantologieinnerhalb der Deutschen Gesellschaft ftir Zahn-, Mundund Kieferheilkunde.Fujioka-Hirai Y, Akagawa Y, Minagi S, Tsuru H, Miyake Y,Suginaka H (1987). Adherence of Streptococcus mutans toimplant materials. Biomed Mater Res 21:913-920.Gristina AG (1987). Biomaterial-centered infection: Microbialadhesion versus tissue integration. Science 237:1588-1595.Joshi RI, Eley A (1988). The in vitro effect of a titaniumimplant on oral microflora: comparision with other metalliccompounds. / Med Microbiol 27:105-107.Kornman KS (1982). Age, supragingival plaque, and steroidhormones as ecological determinants of the subgingivalflora. In: Genco RJ, Mergenhagen SE, editors. Host-parasiteinteractions in periodontal disease. Washington (DC):American Society for Microbiology, 132-138.Lekholm U, Adell R, Lindhe J, Branemark P, Eriksson B,Rockier B, et al. (1986). Marginal tissue reactions atosseointegrated titanium fixtures. Int J Oral MaxillofacSurg 15:53-61.Leonhardt A, Berglundh T, Ericsson I, Dahlen G (1992).Putative periodontal pathogens on titanium implants andteeth in experimental gingivitis and periodontitis in beagledogs. Clin Oral Impl Res 3:112-119.Loesche WJ, Gusberti F, Mettraux G, Higgins T, Syed S(1983). Relationship between oxygen tension andsubgingival bacterial flora in untreated human periodontalpockets. Infect Immun 42:659-667.Mergenhagen SE, Rosan B, editors (1985). Molecular basis oforal microbial adhesion. Washington (DC): AmericanSociety for Microbiology.Mombelli A, Mericske-Stern R (1990). Microbiological featuresof stable osseointegrated implants used as abutments foroverdentures. Clin Oral Impl Res 1:1-7.Mombelli A, Lang NP (1992). Antimicrobial treatment of peri-

206MOMBELUimplant infections. Clin Oral Impl Res 3:162-168.Mombelli A, Van Oosten MAC, Schurch E, Lang NP (1987).The microbiota associated with successful or failingosseointegrated titanium implants. OralMicrobiolImmunol2:145-151.Mombelli A, Buser D, Lang NP (1988). Colonization ofosseointegrated titanium implants in edentulous patients.Early results. Oral Microbiol Immunol 3:113-120.Nakazato G, TsuchiyaH, Sato M, Yamauchi M (1986). In vivoplaque formation on implant materials. IntJOralMaxillofacImplants 4:321-325.Nakou M, Mikx FHM, Oosterwaal PJM, Kruijsen JCWM(1987). Early microbial colonization of permucosal implantsin edentulous patients. J Dent Res 11:1654-1657.Rams TE, Link CC (1983). Microbiology of failing dentalimplants in humans: electron microscopic observations. /Oral Implantol 11:93-100.Rams TE, Roberts TW, Tatum H Jr, Keyes PH (1984). Thesubgingival microbial flora associated with human dentalimplants. J Prosthet Dent 51:529-534.Rams TE, Feik D, Slots J (1990). Staphylococci in humanperiodontal diseases. Oral Microbiol Immunol 5:29-32.Rosenberg ES, Torosian JP, Slots J (1991). Microbialdifferences in 2 clinically distinct types of failures ofosseointegrated implants. Clin Oral Impl Res 2:135-144.Sanz M, Newman MG, Nachnani S, Holt R, Stewart R,Flemmig T (1990). Characterization of the subgingivalmicrobial flora around endosteal sapphire dental implantsin partially edentulous patients. Int J Oral MaxillofacADV DENT RES AUGUST1993Implants 5:247-253.Socransky SS, Haffajee AD, Dzink JL, Hillman JD (1988).Association between microbial species in subgingival plaquesamples. Oral Microbiol Immunol 3:1-7.Ter Steeg PF, Van der Hoeven JS (1990). Growth stimulationof Treponema denticola by periodontal microorganisms.Antonie van Leeuwenhoek 57:63-70.Theilade E, Theilade J (1985). Formation and ecology ofplaque at different locations in the mouth. ScandJDent Res93:90-95.Van Houte J (1982). Colonization mechanisms involved in thedevelopment of the oral flora. In: Genco RJ, MergenhagenSE, editors. Host-parasite interactions in periodontal disease.Washington (DC): American Society for Microbiology,86-97.Van Steenbergen TJM, Van Winkelhoff AJ, De Graaff J(1991). Black-pigmented oral anaerobic rods: Classificationand role in periodontal disease. In: Hamada S, Holt SC,McGhee JR, editors. Periodontal disease: Pathogens & hostimmune responses. Tokyo: Quintessence Publishing Co.,41-52.Wolff LF, Liljemark WF, Pihlstrom BL, Schaffer EM, AeppliDM, Bandt CL (1988). Dark-pigmentedBacteroides speciesin subgingival plaque of adult patients on a rigorous recallprogram. / Periodont Res 23:170-174.Wolinsky LE, de Camargo PM, Erard JC, Newman MG(1989). A study of in vitro attachment of Streptococcussanguis andActinomyces viscosus to saliva-treated titanium.Int J Oral Maxillofac Implants 4:27-31.

BACTERIOLOGY OF THE FAILING IMPLANT The first data on the microbiota associated with unsuccessful implants were presented by Rams and co-workers (Rams and Link, 1983; Rams et al, 1984). These investigators collected samples from 17 implants of various designs (ramus frame

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