Detection of Human Immunodeficiency Virus Antibodies in Oral Fluids

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Clinical and Diagnostic Laboratory Immunology, July 1998, p. 419-426, Vol. 5, No. 4
1071-412X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

MINIREVIEW
Detection of Human Immunodeficiency Virus Antibodies in Oral Fluids

R. L. Hodinka,¹^,²^,^* T. Nagashunmugam,²^,³ and D. Malamud⁴^,⁵

Clinical Virology Laboratory, Departments of Pediatrics and Pathology, Children's Hospital of Philadelphia,¹ Departments of Medicine³ and Biochemistry,⁴ and Schools of Medicine² and Dental Medicine,⁵ University of Pennsylvania, Philadelphia, Pennsylvania 19104

	INTRODUCTION

Top Introduction References

Oral fluids, including saliva, gingival crevicular fluid, and mucosal transudates have been widely used for monitoring drugs,hormones, and a variety of other molecules and chemical substancesfor over 50 years (34, 35, 53, 54, 68). During the pastdecade, the use of oral fluids also has been advocated as a noninvasivealternative to the collection of blood for the detection of antibodiesto a number of specific bacterial (32, 82), viral (1-4, 18,40, 61-65, 75), fungal (41), and parasitic (17, 20) agents.Particular attention has been given to the value of oral fluidsfor the diagnosis of infection with human immunodeficiency virus(HIV) (58, 73).

Oral-fluid testing for HIV antibodies was first reported by Archibald et al. (1-4) and Parry et al. (60, 61). As summarizedby Malamud and Friedman (51), in studies with saliva conductedbetween 1986 and 1991, the concordance between positive serumtests and positive saliva tests for the detection of HIV antibodiesranged from 70 to 100%. The less-than-perfect agreement has ledto considerable confusion regarding the efficacy of using oralfluids in screening for HIV antibody. This is due, in part, tovariations in the type and volume of oral sample collected, howthe sample is handled prior to testing, the concentration of immunoglobulin(Ig) G present, and if testing methods have been modified to accommodatethe use of oral fluids. In early studies that reported poor sensitivity,whole saliva was used and there was little consideration for thevolume and condition of the sample needed and the choice of screeningassays employed. For this reason, investigators have developedspecialized collection devices that enhance the level of antibodies,particularly IgG, in oral specimens, ensure sufficient specimenvolume, and include reagents to prevent microbial growth and proteolyticbreakdown of antibodies. In general, this has been accomplishedby collecting oral fluids enriched in gingival crevicular fluidand mucosal transudate, which possess increased levels of IgGrelative to saliva (46, 66). In addition, recent modificationsto existing HIV antibody assays and the development of extremelysensitive assays specifically designed for oral fluids have greatlyimproved the accuracy of oral-based diagnostic tests for antibodiesto HIV and have compensated for the low levels of antibodies presentin oral secretions compared with serum (46, 66).

In this review, we assess the usefulness of saliva and other oral fluids for the detection of HIV antibodies, discuss thedevices employed for specimen collection, and analyze the currentreliability and accuracy of performing HIV antibody tests on oralsecretions compared to serum or plasma.

	SPECIMEN OF CHOICE

Whole saliva, glandular-duct saliva, or mucosal transudates are specimens that can be collected for tests to detect antibodyto HIV in oral secretions. A basic understanding of these differenttypes of oral fluids, however, is necessary in choosing whichoral fluid is the most appropriate and which method of recoveryis best suited for the testing system employed. Detailed informationon the nomenclature, specimen collection, and immunobiology oforal fluids can be found in references 5, 46, 58, 59,and 66. Best results are obtained with oral fluids that arerich in IgG, since the primary humoral immune response to HIVinfection involves mainly this class of antibodies.

Whole saliva. Whole saliva is the fluid obtained from the mouth by expectoration and includes secretions from the parotid, submandibular,sublingual, and minor salivary glands as well as transudates ofthe oral mucosa. It contains mostly secretory IgA and low levelsof IgG (58). Whole saliva also contains bacteria, leukocytes,mucin, desquamated epithelial cells, and food debris, which maylead to degradation of IgG by bacterial and salivary proteasesand makes the specimen difficult to process due to the viscosity.Either unstimulated saliva or saliva secreted in response to exogenousstimulation can be collected. Unstimulated saliva is obtainedby tilting the head forward and dribbling saliva from the lowerlip into a graduated test tube fitted with a funnel. After 5 min,the subject expectorates any remaining saliva from the mouth.To stimulate saliva, Parafilm, paraffin wax, neutral gum base,or rubber bands can be employed as mechanical stimuli. Dribbledsaliva has a stability of 5 days at room temperature but can bestored for longer times at 4 to $-$ 20°C (63).

Glandular-duct saliva. Saliva from the parotid, submandibular, and sublingual glands is obtained directly from the glandular ducts with speciallydesigned collectors. Absorbent filter paper or suction aspirationwith a micropipette can be used for the collection of secretionsfrom the minor salivary glands. Glandular-duct saliva containspredominantly secretory IgA and should be stored as describedfor whole saliva.

Oral mucosal transudates. Oral mucosal transudates are fluids from the capillaries beneath the buccal mucosa and at the base of the crevice betweenthe teeth and gums. These fluids not only contain secretory IgAbut are rich in IgG and IgM that originate in the plasma and arepassively transferred to the mouth across the mucosa and throughthe gingival crevices. The IgG concentration in oral mucosal transudates,however, is less than that in plasma but higher than that in wholesaliva (46, 66). Thus, a device is required to collect thesefluids in order to efficiently enrich and elute the IgG antibodies;saliva production should not be stimulated during the collection,as this will only decrease the concentration of IgG present inthe final specimen. The terms "crevicular fluid," "gingival crevicularfluid," and "crevicular fluid saliva" also have been used to describeoral mucosal transudates.

	COLLECTION DEVICES

Several devices are commercially available for the collection of oral mucosal transudate specimens for the detection of HIVantibodies (Fig. 1). These include Salivette (Sarstedt Ltd., Leicester,United Kingdom), Orapette (Trinity Biotech, Dublin, Ireland),Omni-SAL (Saliva Diagnostic Systems, Inc., Vancouver, Wash.),and OraSure (Epitope, Inc., Beaverton, Oreg.). The devices aresimple, safe, and convenient to use and provide an adequate homogeneousspecimen with low viscosity. Specimen collection, however, mustbe supervised and the instructions must be carefully followedto ensure specimen adequacy. A transport buffer provided withthe Omni-SAL and Orasure devices contains antimicrobial agentsand protein stabilizers. Specimens may be stored at temperaturesof 4 to 37°C for 21 days or at $-$ 20°C for longer periods (27,72, 78).

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FIG. 1. Commercial devices for the collection of oral-fluid specimens. (A) Salivette; (B) Orapette; (C) Omni-SAL; (D) OraSure.

Salivette. With the Salivette device, a compressed cylinder of cotton is placed in the mouth and is gently chewed for approximately 1min to enhance the release of oral mucosal transudates. The saturatedcotton is then placed inside the provided stoppered inner tubewhich has a small hole in its base. The inner tube fits into anouter tube which possesses a conical base, and oral fluids arecollected by centrifugation.

Orapette. The Orapette device includes a small, rayon ball and a snapped-cap plunger which screws into a receiving container. The rayonball is placed in the mouth, and the subject is asked to concentrateon collecting oral fluids from around the teeth and gum area untilthe rayon is completely saturated. The saturated rayon ball isthen placed into the receiving container, and the plunger is screwedinto the container, compressing the rayon and releasing dropsof oral fluid from a small opening in the container. The fluidis collected in a stoppered tube suitable for transport and testing.

Omni-SAL. The Omni-SAL device employs a compressed, absorbent cotton pad attached to a plastic stem. The pad is placed under the tongueand absorbs fluid from the floor of the mouth. The device incorporatesan indicator on the plastic stem that turns from white to bluewhen an adequate amount of sample has been collected. The collectionpad is then inserted into a stoppered transport tube containing1.1 ml of phosphate-buffered saline, pH 7.0, protease inhibitors,surfactants, antimicrobial agents, and 0.2% sodium azide as apreservative. In the laboratory, the collection pad is compressedand the eluate is filtered with a piston-style filter.

OraSure. The OraSure oral-specimen collection device is the only apparatus that has been licensed by the Food and Drug Administration(FDA) for use in the detection of HIV antibodies in oral fluids.The collection device is available only by order of a physician,and certain restrictions apply to its use. The device is intendedfor subjects 13 years of age and older, it is not to be providedto subjects for home use or to be used to screen blood donors,the use of the device must be administered by properly trainedpersonnel, and test subjects must receive an information pamphletthat explains the limitations of the procedure prior to specimencollection. To obtain the device from the manufacturer, a physicianis required to sign a letter of agreement accepting responsibilityfor the proper training of personnel and use of the collectiondevice, the reporting of test results, and counseling of the subjectabout the results and attesting that specimen collection and HIVantibody testing are done in accordance with laws and regulationsconcerning consent and confidentiality. Training materials andproficiency panels are supplied by the manufacturer to physiciansor laboratories that want to become qualified to collect and testthe oral-fluid specimens.

OraSure uses a flat, absorbent cotton pad which is treated with a salt solution containing 3.5% sodium chloride, 0.3% citricacid, 0.1% potassium sorbate, 0.1% sodium benzoate, and 0.1% gelatin(pH 7.2). The treated pad is then dried, attached to a plastichandle, and packaged for use. For collection of oral specimens,the subject is instructed to place the pad between the lower cheekand gum and to rub back and forth until moist. The pad is thenheld in place for 2 min, removed from the mouth, and placed intoa stoppered transport vial with 0.8 ml of aqueous solution containing0.5% Tween 20 and 0.01% chlorhexidine digluconate as preservatives.Following transport to the laboratory, the fluid is eluted fromthe pad and the eluate is recovered by centrifugation.

Foam swab. Oral-fluid specimens can also be obtained by using a polystyrene foam swab developed at the Public Health Laboratory ServiceVirus Reference Division, London, United Kingdom (63). The tipof the foam swab is similar to a soft sponge and is saturatedwith oral mucosal transudates by rubbing the swab along the junctionof the teeth and gums for approximately 1 min. The oral fluidsare then extracted from the swab into 1 ml of phosphate-bufferedsaline, pH 7.2, containing 0.2% Tween 20 and 10% fetal calf serumand collected by centrifugation (74). This device is not commerciallyavailable.

For each device, a sufficient volume of fluid must be obtained for testing, and this is measured by the laboratory receivingthe specimen or, as with the Omni-SAL device, by using an indicatorof specimen adequacy. Collections typically yield from 0.5 to1.5 ml of oral mucosal transudate. It has been reported by Mortimerand Parry (57) that for 5% of subjects it may be difficult toobtain enough specimen to saturate a collection device becauseof parched mouth. Also, there is no assurance with these devicesthat the appropriate type of fluid and concentration of IgG hasbeen obtained. It has been suggested that IgG levels be determinedfor each specimen prior to testing and that only specimens withat least 0.5 mg of IgG per liter be used (57). Current methodsfor quantifying IgG in oral mucosal transudates, however, arecomplex and insensitive and add time and expense to any screeningsystem for HIV antibody. Also, this may not be necessary withthe development of more sensitive antibody assays. To our knowledge,there have been no published studies that have directly comparedall of the different devices for the collection of oral fluidsfor the detection of HIV antibodies. The cost of using oral-fluidcollection devices is comparable to the expense of collectingblood specimens, while there is little cost involved in the collectionof dribbled whole saliva.

	SCREENING FOR HIV ANTIBODY IN ORAL FLUIDS AND SERUM

Table 1 summarizes the data of 44 studies that compared the use of oral fluids with the use of serum for the detection ofHIV antibodies. We have limited our review to data published infull manuscripts, excluding studies published only as abstracts.The mean sensitivities of oral-fluid-based screening for HIV antibodywere reported to be 95.2% (range, 50 to 100%) for whole salivacompared with 98.6% (range, 92.7 to 100%) for OraSure, 98.1% (range,90.7 to 100%) for Omni-SAL, and 97.9% (range, 88 to 100%) forSalivette. The mean specificities of HIV screening tests withoral-fluid samples were uniformly high: 99.0% (range, 84.1 to100%) for whole saliva, 99.9% (range, 99.2 to 100%) for OraSure,99.7% (range, 98.7 to 100%) for Omni-SAL, and 98.0% (range, 81.8to 100%) for Salivette. Single studies involving Orapette or foamswab collection devices reported sensitivities of 100% for bothsystems and specificities of 99.8 and 100%, respectively. In allreported studies, the sensitivity of oral-fluid testing was measuredby using samples collected from known HIV-seropositive individualsand the specificity was determined with specimens obtained fromindividuals who were at low risk for HIV and were seronegative.

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TABLE 1. Recent studies comparing oral fluids with serum for the detection of antibodies to HIV by screening assays

McAlpine et al. (56) have reported a sensitivity range of 96.9 to 100% and a specificity range of 89.9 to 100% for 13 blood-basedscreening assays for antibodies to HIV, and van Kerckhoven etal. (80) have demonstrated sensitivity and specificity rangesof 96.6 to 100% and 85.6 to 100% for 36 commercial blood-basedassays. A study of six commercial rapid serological tests forHIV-1 antibody conducted by Malone et al. (52) revealed a sensitivitythat ranged from 89.2 to 100% and a specificity ranging from 56.5to 100%. A more recent study by Silvester et al. (69) reportedsensitivity from 99.5 to 99.9% and specificity from 99.5 to 99.9%for four commonly used blood-based enzyme immunoassays that detectantibody to both HIV-1 and HIV-2. Most of the reports in Table1 clearly demonstrate that antibodies to HIV can be detectedin whole saliva and oral mucosal transudate specimens with a sensitivityand a specificity comparable to those of assays which use serum.

The data presented also suggest that the appropriate use of an oral-fluid collection device increases the overall performanceof HIV antibody screening assays compared to the collection ofdribbled whole saliva, although direct comparative studies ofwhole saliva and the various collection devices have not beenaccomplished. This is thought to be due to the increased levelsof IgG in oral mucosal transudates and the use of preservativesin the collection devices to maintain antibody integrity. Cordeiroet al. (14) have reported IgG levels to be 7.2 to >100 mg/literwhen oral fluids are collected with a collection device. Thisis well above the recommended level of 0.5 mg/liter needed toaccurately detect HIV antibody in oral fluids. Also, Gaudetteet al. (27) have demonstrated that preservatives provided withinsome collection devices effectively inhibit microbial overgrowthof collected oral-fluid specimens and maintain the stability ofIgG levels during long-term storage, whereas a marked and progressivedecline in IgG was observed in unpreserved whole saliva. Of thecollection devices for which multiple studies have been performed,use of the OraSure device resulted in the highest reported sensitivitiesand specificities for the detection of HIV antibodies in oralfluids.

A number of different screening assays have been employed for the detection of HIV antibodies in oral fluids (Table 1). Theseinclude both conventional enzyme immunoassays (EIA) and rapidtests designed for use with serum or plasma samples, as well asan IgG antibody capture radioimmunoassay (GACRIA) and enzyme-linkedimmunosorbent assay (GACELISA) optimized for the detection ofHIV antibody in specimens that contain low concentrations of immunoglobulin(12). With screening assays intended primarily for serum orplasma, modifications to the system must be made for oral-fluidspecimens. These have included increasing the sample volume, decreasingthe sample diluent volume, increasing the specimen incubationtime, and lowering the optical density cutoff. When such changesare made and assay protocols are optimized to accept oral-fluidspecimens, the sensitivities and specificities of these assaysare equal to those observed with serum. However, not all blood-basedassays have produced consistent results for oral fluids.

The GACELISA has been used in 17 of the 44 reported studies in Table 1, and highly sensitive and specific results have beenobtained with both whole saliva and specimens obtained with oral-fluidcollection devices. The assay also has demonstrated superiorityto many of the conventional EIA formats, as capturing HIV-specificantibody to a solid phase allows for the enhanced detection oflow levels of HIV antibody in oral-fluid specimens. Recently,Lamey et al. (45) have observed excellent results when usingthe GACELISA on any component of saliva, including not only wholesaliva and oral mucosal transudate but saliva obtained from parotid,submandibular, and minor salivary glands. Testing of oral fluidsby the GACELISA has been shown by Tess et al. (74) to be anaccurate and acceptable method for assessing the HIV infectionstatus of children older than 12 months of age who were born toinfected mothers. Connell and Parry (13) have also shown thatthe GACELISA can detect HIV antibodies in oral fluids at the sametime or within a few days of seroconversion following primaryinfection, whereas other commercial assays may take up to 4 weeksafter seroconversion to detect antibodies in oral fluids. TheGACELISA is manufactured by Murex Diagnostics, Ltd., Dartford,United Kingdom, and is currently available only on the internationalmarket.

The FDA has recently approved a commercial HIV antibody test that is specifically designed for use with oral-fluid specimens.The oral-fluid Vironostika HIV-1 Microelisa system (Organon TeknikaCorporation, Durham, N.C.) has been licensed for use with theassociated OraSure collection device. In two large comparativetrials using this system, sensitivities and specificities of 99.9%were reported by Gallo et al. (26) and 99.2% by Granade et al.(31), respectively. This EIA is identical to the serum-basedVironostika HIV-1 assay, except that the procedure has been modifiedby decreasing the sample dilution from 1 to 75 for serum to 1to 2 for oral fluids. The test system is approved for use in subjects13 years of age and older.

Rapid and simple "point-of-care" tests which use techniques involving membrane capture or particle agglutination have alsobeen used for the detection of HIV antibody in oral fluids. Similarto the conventional EIAs described above, most of these rapidassays were originally designed to be used with serum or plasmabut have been modified to analyze oral-fluid specimens. The performanceof serum-based rapid assays for the detection of HIV antibodyin oral fluids has been reported by many investigators to be excellent(Table 1). In particular, the TestPack HIV-1/HIV-2 (Abbott Laboratories,Abbott Park, Ill.) rapid assay performed exceedingly well, witha sensitivity of 98.6% (range, 95 to 100%) and a specificity of99.9% (range, 99.3 to 100%) in seven published studies. Recently,a prototype oral-fluid-based rapid dipstick assay (OraScreen;Beacon Diagnostics, Foster City, Calif.) was examined by Leowet al. (47) and, when used in combination with the Omni-SALoral-fluid collection device, was found to have a sensitivityof 94.7% and a specificity of 99.5%. The assay consists of a nitrocellulosemembrane spotted with HIV-1 and HIV-2 viral lysates and two referencespots used as a negative control and for the detection of humanIgG antibody. The membrane is reacted with an oral-fluid sample,followed by the addition of a conjugated secondary antibody andsubstrate. The assay is completed in 15 min, and a positive resultis read as a blue-purple dot in the IgG reference and test wells.Saville et al. (67) have recently studied two combinations oforal-fluid collection devices and rapid assays designed specificallyto detect HIV-1 and HIV-2 antibodies in oral fluids. The combinationsof the Orapette collection device with SalivaCard HIV-1/HIV-2assay from Trinity Biotech and the Omni-SAL (Saliva DiagnosticsSystems) collection device with the ImmunoComb II HIV-1 and HIV-2(Orgenics) were shown to be 100% sensitive and 99.8 to 100% specificin testing oral fluids collected from HIV-seropositive and -seronegativeindividuals. The SalivaCard HIV-1/HIV-2 assay involves the chromatographicdiffusion of sample, enzyme-conjugated secondary antibody, andsubstrate along a solid matrix coated with synthetic HIV peptides.Interaction of HIV-specific antibodies with the peptide antigensresults in a blue color of an intensity equal to or greater thanthat of a provided control. The assay is completed in 12 min.The ImmunoComb II HIV-1 and HIV-2 assay incorporates a plasticcomb with 12 projections which are sensitized in three separatespots with either HIV-1 or HIV-2 synthetic peptides or goat antibodiesto human IgG as an internal control. By using a modified dipsticktechnique, the projections are placed in a developing plate thatcontains six rows of 12 wells each; samples of oral fluids areplaced in the first row of 12 wells, and each subsequent row of12 wells contains a different reagent used for the next step ofthe assay. The comb is moved from row to row with incubationsat each step, and the results are read as a gray-blue spot onthe projections of the comb indicating the detection of antibodyto HIV-1 or HIV-2 and the presence of human IgG antibody boundto the control spot. A total of 10 specimens and two controlscan be tested in approximately 35 min with this method. The mainadvantages of using rapid assays for the detection of HIV antibodyin oral fluids are speed, simplicity, and convenience. The performanceof these assays requires limited laboratory resources and trainingof personnel, and many of the assays are formatted to includebuilt-in quality controls. Unlike conventional EIAs, they alsocan be performed without electricity and sophisticated equipment,which may be unavailable in developing countries and under certaintesting situations in the field. In conjunction with an appropriateoral-fluid collection device, certain rapid assays have demonstrateda degree of sensitivity and specificity for the detection of HIVantibody comparable to those for serum.

	CONFIRMATORY TESTING

Available data on the use of Western blot techniques to confirm the presence of HIV antibody in whole saliva and oral-fluidspecimens collected with various devices are summarized in Table2. The performance of confirmatory Western blots on oral-fluidspecimens was initially problematic, with many indeterminate andnegative reactivities compared to results for matched serum specimens.Although reactivities to the HIV-1 envelope proteins gp160 andgp120 were observed for most oral-fluid specimens, other HIV-specificproteins were not seen with any consistency. Larger specimen volumeswere also necessary to compensate for the loss of Western blotsensitivity, but adequate volumes were not always available forall oral-fluid specimens. Modifications in the chemistry and proceduresof both commercial and in-house standard Western blot methods,however, have allowed for efficient and accurate detection ofantibodies to HIV-1 in oral fluids by Western blot. In particular,Granade et al. (30) have developed an in-house miniaturizedWestern blot assay that has been optimized by decreasing the specimendilution and increasing the specimen and conjugate incubationtimes. This technique requires much smaller specimen volumes thanthose used in conventional Western blot procedures, and specimendilution is minimized so as not to decrease the IgG concentrationin the oral fluids.

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TABLE 2. Recent studies comparing oral fluids with serum for the confirmation of antibodies to HIV by Western blot

A confirmatory test for oral-fluid specimens has been approved by the FDA. The OraSure HIV-1 Western blot kit (Epitope Inc.)is a modification of the manufacturer's Western blot assay forserum and has been licensed for use with oral-fluid specimenscollected with the OraSure collection device and that are foundto be repeatedly reactive by the oral-fluid Vironostika HIV-1Microelisa system. Gallo et al. (26) recently demonstrated thatthis Western blot procedure has a sensitivity and a specificitycomparable to those obtained for matched serum specimens for HIVantibody. The sensitivity of this assay was achieved by decreasingthe specimen dilution from 1 to 51 for serum to 1 to 7.7 for oralfluids, increasing the incubation of specimens with Western blotstrips from 1 h to 3 h, and using a highly sensitive enzyme-substratecombination as part of the antibody detection strategy.

	APPLICATIONS

There are many advantages to using oral fluids instead of serum or plasma specimens in serological assays for antibodies toHIV. The collection of oral fluids is rapid and less invasiveand does not require laboratory personnel with special training;patients can easily obtain the samples themselves. Collectionof oral-fluid specimens also increases compliance (7, 11,50) and alleviates the fear that patients may experience whenhaving their blood drawn. It reduces the potential danger to thehealth professional through blood exposure and provides a safersample to handle since saliva and oral fluids have been shownto inactivate HIV and possess less infectious virus than blood(51, 85). The use of oral fluids in screening for HIV antibodymay also benefit more challenging populations whose blood maybe difficult to obtain, including children, hemophiliacs, obesepeople, and the elderly and infirm, and may permit improved accessfor the surveillance of intravenous drug users, homeless persons,sex industry workers, and persons in developing countries. Ithas also been shown that recent food intake, dentition, poor oralhygiene, gingivitis, periodontitis, oral ulcers, tobacco consumption,and the use of anticholinergic drugs have no effect on test resultsfor oral-fluid specimens (6, 19) and that oral-fluid testingis not affected by conditions known to be associated with increasedfrequency of false-positive blood-based HIV test results, suchas autoimmune disease, multiple births, other viral infections,or polyclonal or monoclonal gammopathy (26). Finally, the useof oral fluids may afford a greater opportunity to screen forHIV antibodies in physicians' and dentists' offices, point-of-caresettings, public health institutions, and community outreach programs.Although oral-fluid-based testing for HIV antibody has been suggestedfor home use, collection devices and antibody assays have notbeen approved for this purpose.

	SPECIFIC ISSUES AND FUTURE CONSIDERATIONS

We have reviewed the use of oral fluids and the performance of a variety of serological assays for the detection and confirmationof HIV antibody and conclude that testing of oral fluids is aviable alternative to blood for the detection of antibodies toHIV. Although earlier studies showed inconsistent results withless than optimum sensitivity and specificity, results of morerecent work are far more encouraging. With an adequate collectionof oral fluids and an appropriate choice of antibody assays, testingof oral-fluid specimens is as accurate as screening blood forHIV antibody.

As with screening and confirmatory assays designed for the detection of HIV antibodies in serum or plasma, testing technologiesand strategies using oral fluids continue to evolve. Developedprocedures for specimen collection and testing of oral fluidsrequire further improvement and standardization, and appropriatequality assurance programs must be established for use of oralfluids. Direct comparisons of the various oral-fluid collectionmethods are needed to better determine their reliability, appropriateness,ease of use, and cost. More research is also necessary to developtesting strategies and algorithms for use with oral fluids thatcomply with the accepted standards used for blood testing andto define testing situations where the use of oral fluids is themost appropriate. It would appear that it is only a matter oftime before standard protocols are established and implementedfor the use of oral fluids in donor screening, monitoring populationsfor the prevalence of HIV, diagnosing HIV infection, and research.

	ACKNOWLEDGMENTS

This work was supported in part by grants from the National Institutes of Health (DE 09569) and World Health Direct.

	FOOTNOTES

^* Corresponding author. Mailing address: Children's Hospital of Philadelphia, 34th and Civic Center Blvd., Philadelphia, PA19104. Phone: (215) 590-2028. Fax: (215) 590-2556. E-mail: hodinka{at}email.chop.edu.

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MINIREVIEW Detection of Human Immunodeficiency Virus Antibodies in Oral Fluids

MINIREVIEW
Detection of Human Immunodeficiency Virus Antibodies in Oral Fluids