Co-infections of adenovirus species in previously vaccinated patients.Despite the success of the adenovirus adenovirus Any of a group of spheroidal viruses, made up of DNA wrapped in a protein coat, that cause sore throat and fever in humans, hepatitis in dogs, and several diseases in fowl, mice, cattle, pigs, and monkeys. vaccine administered to US military trainees, acute respiratory disease Noun 1. respiratory disease - a disease affecting the respiratory system respiratory disorder, respiratory illness adult respiratory distress syndrome, ARDS, wet lung, white lung - acute lung injury characterized by coughing and rales; inflammation of the (ARD Ard (ärd), in the Bible. 1 Son of Benjamin. 2 Benjamite, perhaps the same as (1.) An alternate form is Addar. ) surveillance still detected breakthrough infections (respiratory illnesses Noun 1. respiratory illness - a disease affecting the respiratory system respiratory disease, respiratory disorder adult respiratory distress syndrome, ARDS, wet lung, white lung - acute lung injury characterized by coughing and rales; inflammation of the associated with the adenovirus serotypes specifically targeted by the vaccine). To explore the role of adenoviral co-infection (simultaneous infection by multiple pathogenic path·o·gen·ic or path·o·ge·net·ic adj. 1. Having the capability to cause disease. 2. Producing disease. 3. Relating to pathogenesis. adenovirus species) in breakthrough disease, we examined specimens from patients with ARD by using 3 methods to detect multiple adenoviral species: a DNA microarray DNA microarray A small solid support, usually a membrane or glass slide, on which sequences of DNA are fixed in an orderly arrangement. DNA microarrays are used for rapid surveys of the expression of many genes simultaneously, as the sequences contained on a , a polymerase chain reaction polymerase chain reaction (pŏl`ĭmərās') (PCR), laboratory process in which a particular DNA segment from a mixture of DNA chains is rapidly replicated, producing a large, readily analyzed sample of a piece of DNA; the process is (PCR PCR polymerase chain reaction. PCR abbr. polymerase chain reaction Polymerase chain reaction (PCR) )--enzyme-linked immunosorbent immunosorbent /im·mu·no·sor·bent/ (-sor´bent) an insoluble support for antigen or antibody used to absorb homologous antibodies or antigens, respectively, from a mixture; the antibodies or antigens so removed may then be eluted in pure assay, and a multiplex See multiplexing. PCR assay. Analysis of 52 samples (21 vaccinated, 31 unvaccinated) collected from 1996 to 2000 showed that all vaccinated samples had co-infections. Most of these coinfections were community-acquired serotypes of species B1 and E. Unvaccinated samples primarily contained only 1 species (species E) associated with adult respiratory illness. This study highlights the rarely reported phenomenon of adenoviral co-infections in a clinically relevant environment suitable for the generation of new recombinational variants. ********** Adenoviruses cause an estimated 8% of clinically relevant viral disease globally (1). Human adenoviruses (HAdVs) are divided into 51 serotypes (HAdV-1 HAdV-51) on the basis of type-specific antiserum-mediated neutralization neutralization, chemical reaction, according to the Arrhenius theory of acids and bases, in which a water solution of acid is mixed with a water solution of base to form a salt and water; this reaction is complete only if the resulting solution has neither acidic nor of infectivity infectivity ability of an agent to infect. (determined primarily by the hexon coat protein and terminal knob portion of the fiber protein) (2) and into 6 species, also referred to as subgenera or subgroups (HAdV-A, B, C, D, E, and F) on the basis of hemagglutination hemagglutination /he·mag·glu·ti·na·tion/ (he?mah-gloo-ti-na´shun) agglutination of erythrocytes. he·mag·glu·ti·na·tion n. inhibition and biochemical criteria (3-5). Species HAdV-B is further classified into subspecies subspecies, also called race, a genetically distinct geographical subunit of a species. See also classification. B1 and B2 (3). In civilian populations, HAdV-B1 serotypes 3, 7, 16, and 21; HAdV-E serotype serotype /se·ro·type/ (ser´o-tip) the type of a microorganism determined by its constituent antigens; a taxonomic subdivision based thereon. se·ro·type n. See serovar. v. 4; and 1 member of subspecies HAdV-B2, serotype 14, cause outbreaks of illness ranging from mild febrile febrile /feb·rile/ (feb´ril) pertaining to or characterized by fever. feb·rile adj. Of, relating to, or characterized by fever; feverish. respiratory infections Noun 1. respiratory infection - any infection of the respiratory tract respiratory tract infection infection - the pathological state resulting from the invasion of the body by pathogenic microorganisms and conjunctivitis conjunctivitis (kənjəngtəvī`təs), inflammation or infection of the mucosal membrane that covers the eyeball and lines the eyelid, usually acute, caused by a virus or, less often, by a bacillus, an allergic reaction, or an to potentially lethal disseminated infections in both adults and children (1, 6). HAdV-C serotypes 1, 2, 5, and 6 cause locally endemic upper respiratory infections Noun 1. upper respiratory infection - infection of the upper respiratory tract respiratory infection, respiratory tract infection - any infection of the respiratory tract in infants and children (7,8) and occasional outbreaks in adults. Other HAdV species are usually not associated with respiratory disease in otherwise healthy humans. HAdV seems to have found a particularly destructive niche in military training camps. HAdV-B1 serotypes 3, 7, and 21; HAdV-E serotype 4; and HAdV-B2 serotype 14 have caused severe outbreaks of acute respiratory disease (ARD) among military recruits in training centers (9,10). Before initiation of an HAdV vaccination program in 1971, outbreaks occurred regularly, and [approximately equal to] 1 of 6 recruits in affected camps required hospitalization hospitalization /hos·pi·tal·iza·tion/ (hos?pi-t'l-i-za´shun) 1. the placing of a patient in a hospital for treatment. 2. the term of confinement in a hospital. (1). Systematic vaccination of recruits against the 2 most common agents of ARD in the military, HAdV serotypes 4 and 7, decreased HAdV-specific respiratory illness by 95% to 99% and overall respiratory illness rates by 50% to 60% (11-13). Despite this general efficacy, breakthrough infection (infection of vaccinated persons by the vaccine-targeted adenoviral serotypes) was still regularly reported (14). Production of the vaccine was suspended in 1996, at which point vaccination became sporadic until the existing stocks ran out in 1999. ARD rates quickly returned to prevaccine levels, with HAdV as the apparent causal agent Noun 1. causal agent - any entity that produces an effect or is responsible for events or results causal agency, cause physical entity - an entity that has physical existence . As a result, reintroduction Noun 1. reintroduction - an act of renewed introduction intro, introduction, presentation - formally making a person known to another or to the public of the vaccine is being actively pursued (15). To explore the possibility that unique HAdV strains were causing ARD in vaccinated persons, throat swab samples were selected from the Naval Health Research Center population-based febrile respiratory illness surveillance collection from vaccinated (n = 21) and unvaccinated (n = 31) recruits who reported ARD from 1996 to 2000. Samples were chosen that had tested positive for serotypes 4 or 7 by culture and serotypic antibody neutralization. The gene coding for the primary adenoviral antigen, the hexon coat protein, was sequenced from these isolates. The sequence data suggested that the detectable serotype 4 and 7 strains apparently responsible for breakthrough infection were the same as those circulating in unvaccinated military and civilian populations (16). In this study, we reanalyze the same set of samples to identify co-infections with multiple HAdV strains and to address what role co-infections may play in breakthrough infection. Materials and Methods Sample Collection and Preparation Samples were collected as throat swabs into viral transport medium from military recruits with ARD at a variety of training camps as previously described (16). The throat swab samples were cultured on A549 cells A549 cells are human alveolar basal epithelial cells. A549 cells fall under the squamous subdivision of epithelial cells, associated with the diffusion of water, electrolytes, and other substances. and tested by using standard serologic se·rol·o·gy n. pl. se·rol·o·gies 1. The science that deals with the properties and reactions of serums, especially blood serum. 2. methods. Both original swabs and in vitro in vitro /in vi·tro/ (in ve´tro) [L.] within a glass; observable in a test tube; in an artificial environment. in vi·tro adj. In an artificial environment outside a living organism. tissue culture fluid (ITCF ITCF Integration, Test, and Control Facility ) samples were stored at -80[degrees]C. Samples that initially tested positive for serotypes 4 or 7 by culture and microneutralization were chosen for analysis and grouped by previous vaccination status. DNA DNA: see nucleic acid. DNA or deoxyribonucleic acid One of two types of nucleic acid (the other is RNA); a complex organic compound found in all living cells and many viruses. It is the chemical substance of genes. extracts from ITCF samples were collected and used in molecular assays. Collection details and symptom definitions were previously reported (16), and sample details are shown in Tables 1 and 2. Initially, 13 unidentified (blinded) samples were sent by the Naval Health Research Center to the Naval Research Laboratory Noun 1. Naval Research Laboratory - the United States Navy's defense laboratory that conducts basic and applied research for the Navy in a variety of scientific and technical disciplines NRL personnel for testing. After the initial 13 samples showed a high rate of respiratory HAdV co-infection, primarily in vaccinated persons, an additional 39 samples were tested in an unblinded fashion. Microarray-based Genotyping Genotyping refers to the process of determining the genotype of an individual with a biological assay. Current methods of doing this include PCR, DNA sequencing, and hybridization to DNA microarrays or beads. One microliter microliter /mi·cro·li·ter/ (µL) (mi´kro-le?ter) one millionth (10-6) of a liter. mi·cro·li·ter n. A unit of volume equal to one-millionth (10-6) of a liter. of purified DNA extract from each of the 52 ITCF samples was used as the template in 50-[micro]L degenerate degenerate /de·gen·er·ate/ (de-jen´er-at) to change from a higher to a lower form. degenerate /de·gen·er·ate/ (de-jen´er-at) characterized by degeneration. PCR amplifications targeting portions of the E1A, hexon, and fiber genes. The primers, degenerate polymerase chain reaction (PCR) amplification protocol, probes, and microarray See micro array. microarray - A technique for performing many DNA experiments in parallel. Nothing to do with computers. fabrication fabrication (fab´rikā´sh  n),n the construction or making of a restoration. techniques have been previously described (18). Once constructed, the spotted microarrays were blocked with a 3% bovine serum albumin-casein solution (BSA-C) for 15 min at room temperature, and the slides were outfitted with MAUI Mixer DC hybridization hybridization /hy·brid·iza·tion/ (hi?brid-i-za´shun) 1. crossbreeding; the act or process of producing hybrids. 2. molecular hybridization 3. chambers (BioMicro Systems, Salt Lake City, UT, USA). Twenty-microliter hybridization reactions (13.6 [micro]L biotinylated degenerate PCR amplicons, 2 [micro]L 3% BSA-C, 4 [micro]L 20x SSC SSC Secondary School Certificate SSC Standard Systems Center (USAF) SSC State Services Commission (New Zealand) SSC Swedish Space Corporation SSC Salem State College (Massachusetts) (0.3 mol/L sodium citrate sodium citrate n. A white crystalline or granular compound, Na3C6H5O7·2H2O, used in photography and in medicine especially as an anticoagulant of blood stored for transfusion. , 3.0 mol/L NACl, pH 7.0), and 0.4 [micro]L 10% sodium dodecyl sulfate Sodium dodecyl sulfate (or sulphate) (SDS or NaDS) (C12H25NaO4S),is an anionic surfactant that is used in household products such as toothpastes, shampoos, shaving foams and bubble baths for its thickening effect and its ability to [SDS 1. (company) SDS - Scientific Data Systems. 2. (tool) SDS - Schema Definition Set. ]) were denatured de·na·ture tr.v. de·na·tured, de·na·tur·ing, de·na·tures 1. To change the nature or natural qualities of. 2. for 3 min at 98[degrees]C and immediately applied to the microarrays. Hybridizations were performed for 2 h at 63[degrees]C in a MAUI Hybridization System (BioMicro Systems). Slides were then washed twice with 4x SSC-0.2% SDS buffer and 2x SSC buffer, and hybridization was detected by the sequential addition of Cy5-conjugated mouse antibiotin immunoglobulin G immunoglobulin G n. Abbr. IgG The most abundant class of antibodies found in blood serum and lymph and active against bacteria, fungi, viruses, and foreign particles. Immunoglobulin G antibodies trigger action of the complement system. (IgG) (Jackson ImmunoResearch, West Grove, PA, USA) and Cy5-conjugated goat antimouse IgG (Jackson ImmunoResearch). Images were obtained with a ScanArray Lite confocal confocal see confocal microscopy. laser scanning system (Perkin-Elmer, Torrance, CA, USA) at a laser power of 60 to 80 and a photomultiplier tube A vacuum tube that converts light into electrical energy and amplifies it. Photomultiplier tubes are used in high-end drum scanners, because they are more sensitive to light than the CCD elements used in lower-cost devices. gain of 60 to 80. The fluorescent signal from each microarray element was considered positive only when its quantified intensity was >3x that of known internal negative control elements. Each ITCF sample was subjected to 2 to 5 independent amplification and hybridization experiments. Hybridization patterns unique to specific serotypes were determined empirically with prototype strains (18). Although members of species HAdV-B1 often produced complex hybridization profiles (18), these profiles were unique, reproducible, and readily identifiable in both single infections and co-infections. Adenovirus Consensus PCR--Enzyme-linked Immunosorbent Assay We used a commercially available kit capable of typing adenoviruses to the species level to confirm the results obtained with microarray analyses. Briefly, the Adenovirus Consensus kit (Argene, North Massapequa, NY, USA) uses a PCR--enzyme-linked immunosorbent assay that amplifies a fragment from the adenovirus virus-associated (VA) RNA RNA: see nucleic acid. RNA in full ribonucleic acid One of the two main types of nucleic acid (the other being DNA), which functions in cellular protein synthesis in all living cells and replaces DNA as the carrier of genetic gene and subsequently detects and types the amplicon with species-specific biotinylated oligonucleotide Oligonucleotide A deoxyribonucleic acid (DNA) or ribonucleic acid (RNA) sequence composed of two or more covalently linked nucleotides. Oligonucleotides are classified as deoxyribooligonucleotides or ribooligonucleotides. probes in a colorimetric col·or·im·e·ter n. 1. Any of various instruments used to determine or specify colors, as by comparison with spectroscopic or visual standards. 2. microwell format (19). Results obtained with the kit were interpreted according to according to prep. 1. As stated or indicated by; on the authority of: according to historians. 2. In keeping with: according to instructions. 3. the manufacturer's adenovirus typing protocol. Adenovirus-specific PCR The species-specific PCR amplification was performed with previously published primers (20) and a Multiplex PCR Kit (Qiagen, Valencia, CA, USA) according to the manufacturer's instructions (with 0.5x Q solution). These amplifications were performed in 25-[micro]L reaction volumes at an annealing annealing (ənēl`ĭng), process in which glass, metals, and other materials are treated to render them less brittle and more workable. temperature of 52[degrees]C. In general, the PCRs were performed in an iCycler (Bio-Rad, Hercules, CA, USA) and analyzed by electrophoresis electrophoresis (ĭlĕk'trōfərē`sĭs): see colloid. electrophoresis Movement of electrically charged particles in a fluid under the influence of an electric field. on 1.5% agarose agarose more highly purified form of agar with similar uses to agar and widely used in the separation of nucleic acid fragments. gels. Monoplex PCR was performed under identical reaction conditions, except that the same primers were used in independent reactions. Sequencing reactions and microneutralization assays were performed as previously described (21,22). Serotype-specific PCR assays (Tables 1 and 2) were verified as described (20,23-26), with occasional substitutions of polymerase type and annealing temperature adjustments. Co-infection Separation Limiting dilutions of ITCF sample 7151 were plated on A549 cells and allowed to adsorb adsorb /ad·sorb/ (ad-sorb´) to attract and retain other material on the surface; to conduct the process of adsorption. ad·sorb v. To take up by adsorption. for 16 hours, after which agarose overlays (0.4% agarose in Dulbecco minimal essential medium, 2% fetal bovine serum Fetal bovine serum ( or foetal bovine serum) is serum taken from the fetuses of cows. Fetal Bovine Serum (or FBS) is the most widely used serum in the culturing of cells. In some papers the expression foetal calf serum is used. , 4 mmol/L glutamine glutamine (gl  `təmēn), organic compound, one of the 20 amino acids commonly found in animal proteins. ) were added to each infected monolayer mon·o·lay·ern. 1. A film or layer one molecule thick formed at the interface between water and either oil or air by a substance such as a partially esterified fatty acid that contains both hydrophobic and hydrophilic groups in the same . Well-separated virus plaques were picked 5 days postinfection, placed into viral transport medium, and tested by PCR for HAdV-B and HAdV-C. A second round of plaque purification was performed on several plaque isolates that were treated with 0.05% Triton-X 100 to potentially disrupt virus clumps clump n. 1. A clustered mass; a lump: clumps of soil. 2. A thick grouping, as of trees or bushes. 3. A heavy dull sound; a thud. v. before their dilution and plating. After 6 hours of adsorption adsorption, adhesion of the molecules of liquids, gases, and dissolved substances to the surfaces of solids, as opposed to absorption, in which the molecules actually enter the absorbing medium (see adhesion and cohesion). , the original inoculum inoculum /in·oc·u·lum/ (-ok´u-lum) pl. inoc´ula material used in inoculation. in·oc·u·lum n. pl. was removed, and the monolayers were overlayed with agarose solution. The newly formed plaques were tested as described above. Results By using a new 70-mer spotted microarray (18), a PCR-enzyme-linked immunosorbent assay (19), and a species-specific multiplex PCR assay (20), we generated data profiles for each of the 52 tissue culture-amplified samples; the raw data from 2 of these samples are shown as representative examples (Figure). The microarray profile of vaccinated sample 7274 detected HAdV-4 (species E), HAdV-21 (species B1), HAdV-C, and HAdV-B2 according to previously validated hybridization patterns (18) (Figure, panel A). Except for detection of an apparent low-level HAdV-C co-infectant, the results of the Adenovirus Consensus kit (HAdV-B1, HAdV-B2, and HAdV-E) (Figure, panel B), multiplex and monoplex species-specific PCR (HAdV-B and HAdV-E) (Figure, panel C), and serotype-specific PCR (HAdV-4, HAdV-21, and HAdVB2) (Figure, panel D) confirmed the microarray-based identification of multiple adenoviral strains in sample 7274. In contrast, the microarray profile of unvaccinated sample 10756 detected a single serotype, HAdV-4 (Figure, panel E). The microarray-based finding was verified by results of the Adenovirus Consensus kit (Figure, panel F), multiplex species-specific PCR (Figure, panel G), and HAdV-4 serotype-specific PCR (Figure, panel H). The data profiles for all 52 samples assembled and compared in this manner are shown in Tables 1 and 2. Dual, triple, and quadruple quad·ru·ple adj. 1. Consisting of four parts or members. 2. Four times as much in size, strength, number, or amount. 3. Music Having four beats to the measure. n. infections were found in all 21 of the vaccinated samples and in 14 of the 31 unvaccinated samples tested (Tables 1 and 2). Previously vaccinated persons showed a high rate of co-infection with both species commonly associated with ARD (HAdV-B1 and HAdV-E), whereas unvaccinated persons were primarily infected with HAdV-E. Since HAdV-4 and HAdV-7 are the 2 most common ARD-associated serotypes, that they were also the most commonly paired respiratory pathogenic co-infectants detected in vaccinated persons is not surprising. When the vaccine was used, the rates of other respiratory adenoviruses were much higher than when the vaccine was not used (16). However, these isolates were chosen for study because they yielded antigenic signals consistent with either HAdV-4 or HAdV-7 and were therefore expected to contain at least 1 of these 2 viruses as the highest titer titer /ti·ter/ (ti´ter) the quantity of a substance required to react with or to correspond to a given amount of another substance. adenoviral components (Table 1) (16). The ability of the microarray to identify to the serotype level resulted in the detection of the greatest number of co-infections, despite its inability to detect members of species B2 when a co-infecting HAdV-7 was present (hybridization pattern interference) and members of species F that were not targeted (Table 3). Microarray-based identification of multiple ARD-associated serotypes from diverse HAdV-B1 species (serotypes 3, 7, and 21) was necessary because co-infections with these serotypes would not have been indicated or resolved by methods limited to species-level identification. Although most apparent co-infections could be verified by each of the primary methods tested and by serotype-specific PCR (e.g., single infections: 10756, 60406, 20142; co-infections: 1212, 7151, 7274), some could not be verified (e.g., 60691, CHPPM CHPPM Center for Health Promotion and Preventive Medicine (US Army) 2). Those co-infectant signals that could not be verified were usually weak positives. The strains responsible for these signals appeared to be subordinate co-infectants because the predominant serotype or species signals generated for the associated samples by the microarray, Adenovirus Consensus kit, and serotype-specific PCR were corroborated cor·rob·o·rate tr.v. cor·rob·o·rat·ed, cor·rob·o·rat·ing, cor·rob·o·rates To strengthen or support with other evidence; make more certain. See Synonyms at confirm. in every case and matched the results obtained from the sequencing experiments previously reported (16). The microarray and Adenovirus Consensus kit use detection and signal amplification techniques that enhance assay sensitivity Assay sensitivity is a property of a clinical trial defined as the ability to distinguish an effective treatment from a less effective or ineffective treatment. Without assay sensitivity, a trial cannot be said to make a distinction between the efficacy of two treatments. and thus render them more sensitive than traditional PCR/agarose gel visualization techniques, as shown by the number of triple and quadruple co-infections detected with these techniques (Table 3). Thus, attempting to corroborate To support or enhance the believability of a fact or assertion by the presentation of additional information that confirms the truthfulness of the item. The testimony of a witness is corroborated if subsequent evidence, such as a coroner's report or the testimony of other these methods with the 3 PCR-based methods used was not completely successful. Nevertheless, most of the positive results from these tests were verified by comparing the microarray and Adenovirus Consensus kit results or by comparison with the results from independent methods such as microneutralization, hexon sequence analysis, serotype-specific PCR that uses primers not used in the multiplex tests, and PCR amplicon sequencing (Tables 1, 2, and 4). These results suggest that these methods can identify and corroborate HAdV co-infections and that, in general, the HAdV load in ARD patients is more complex than previously thought. To determine whether >1 replication-competent serotype or strain was present in the samples with evidence of co-infection, we attempted to physically separate the paired co-infectants in sample 7151 by plaque purification. Of 92 plaques picked from the initial plate, all tested positive for HAdV-C by PCR and 12 of 92 also tested positive for HAdV-B. Several of the plaques that retained both HAdV-B and HAdV-C signals were replaqued, and PCR testing of these plaques yielded only HAdV-C isolates. Further efforts that used a detergent detergent (dētûr`jənt, dĭ–), substance that aids in the removal of dirt. Detergents act mainly on the oily films that trap dirt particles. to increase separation within the original ITCF sample 7151 and applied the agarose overlay more quickly (6 hours) to prevent interplaque contamination also yielded only HAdV-C plaques (data not shown). Discussion We demonstrate the rarely reported phenomenon of co-infections with multiple adenoviral species. Two previous studies have noted rare instances of HAdV-C dual infections in small numbers (27,28). HAdV-C, although rarely associated with pharyngitis pharyngitis Inflammation and infection (usually bacterial or viral) of the pharynx. Symptoms include pain (sore throat, worse on swallowing), redness, swollen lymph nodes, and fever. outbreaks in recruits (10), is usually seen in children (7,8) and can produce latent infections that last into young adulthood. This fact, combined with low incidence of co-infection (27,28), has led to the assertion that multistrain adenovirus co-infections are not common (28) or clinically relevant. The results from the population tested in this study suggest otherwise. Samples from vaccinated recruits showed a high rate of co-infection with multiple species of adenovirus associated with adult ARD (HAdV-E and HAdV-B1). Many of the identified co-infectants in this study were species not generally associated with ARD in the military (HAdV-C, HAdV-B2, and HAdV-F). Although these species were not likely the cause of ARD observed in these patients, since they are not believed to cause ARD in adults and because they have a high potential for latent carriage (1,7,8,29), their presence sheds new light on the general complexity of the human adenoviral load. In addition, they remain viable reservoirs capable of genetic complementation Complementation (genetics) The complementary action of different genetic factors. The term usually implies two homologous chromosomes or chromosome sets, each defective because of mutation and unable by itself to promote the normal development or metabolism of or recombination recombination, process of "shuffling" of genes by which new combinations can be generated. In recombination through sexual reproduction, the offspring's complete set of genes differs from that of either parent, being rather a combination of genes from both parents. with upper respiratory strains. Recombination can generate new strains with unique and stable phenotypes. Intraspecies in·tra·spe·cif·ic also in·tra·spe·cies adj. Arising or occurring within a species: intraspecific competition. Adj. 1. adenovirus recombination has been demonstrated in laboratory cell-culture co-infection studies (30-32). These recombination events can generate viable hybrids with intermediate or unique immunogenic im·mu·no·gen·ic adj. Producing an immune response. immunogenic producing immunity; evoking an immune response. and tropic properties. Evidence suggests recombination can generate hybrids in immunocompromised immunocompromised /im·mu·no·com·pro·mised/ (-kom´pro-mizd) having the immune response attenuated by administration of immunosuppressive drugs, by irradiation, by malnutrition, or by certain disease processes (e.g., cancer). patients (29,33,34), possibly as a result of co-infection with normally isolated serotypes. Recombination, particularly intraspecies, seems to play a major role in the evolution of new, virulent vir·u·lent adj. 1. Extremely infectious, malignant, or poisonous. Used of a disease or toxin. 2. Capable of causing disease by breaking down protective mechanisms of the host. Used of a pathogen. 3. strains of HAdV (1,17,35,36). The currently dominant pathogenic HAdV in US military recruits, a considerably diverged variant HAdV-4 strain (16), appears to be a recent recombinant between HAdV-4 and an HAdV-B1 serotype, probably HAdV-7 (3 7). Given that these 2 are the most common co-infectants seen in our sample set, this finding suggests that the observed dominance of co-infections in vaccinated persons may have contributed to the emergence of the new variant. In general, the understanding and control of situations that create or promote co-infection may be important considerations. The HAdV vaccine, an enteric-coated live-virus tablet designed to transiently and selectively infect the gastrointestinal tract gastrointestinal tract n. The part of the digestive system consisting of the stomach, small intestine, and large intestine. Gastrointestinal tract with normal respiratory HAdV strains, contains viable HAdV-4 and HAdV-7. Thus, we cannot assume whether the detected co-infectants arose from the vaccine itself or from community acquisition of circulating strains. Most HAdV-4 strains in this study are not the vaccine strain but rather a highly divergent variant that has recently been dominant in military training centers (GenBank strain Z-G 95-873). This identity was shown by sequence analysis of 1,500 bp of the hexon gene from many primary infectants identified in the same sample set that was analyzed here (16). The variant HAdV-4 isolates consistently differ from the vaccine strain by 32 base substitutions, including 9 coding changes, in this region (16) (Table 1). Hexon sequence analysis showed that many HAdV-7 co-infectants are HAdV-7d2. HAdV-7d2 is distinguished from the HAdV-7 vaccine strain (HAdV-7a) by a single coding polymorphism polymorphism, of minerals, property of crystallizing in two or more distinct forms. Calcium carbonate is dimorphous (two forms), crystallizing as calcite or aragonite. Titanium dioxide is trimorphous; its three forms are brookite, anatase (or octahedrite), and rutile. in the hexon sequence, but this polymorphism (protein L443Q or nucleotide nucleotide (n `klēətīd', ny`–), organic substance that serves as a monomer in forming nucleic acids. Tl 328A in
GenBank [16]) is specific to HAdV-7d and HAdV-7d2 and is not found in
HAdV-7a, b, c, g, or h or in the vaccine strain (16,38,39). Three of the
other HAdV-7 co-infectants (1856, 4185, and 7372) were shown to be
HAdV-7h by fiber gene sequencing. The fiber gene of HAdV-7h appears to
have been horizontally transferred from HAdV-3 and thus is highly
diverged from the usual HAdV-7 fiber gene, as found in the vaccine
strain (1 7). Thus, sequence analyses show that most, if not all,
co-infectants are currently circulating HAdV-4 and HAdV-7 strains that
are distinct from the vaccine strains (16) (Table 1).Four lines of evidence support the idea that most of the apparent genetic complexity in the throat swab samples comes from multiple strains, as opposed to recombinants with mixed genetic characteristics. The first comes from the microarray data. The microarray tests for hybridization of 6 independent probes designed to match serotype-specific sequences in 3 genes (18). Since different species do not cross-react among the microarray probes, hybridization of genes from 1 species to the identifying probes for 2 species would require redundant presence of 2 different alleles in all 3 genes. Since both natural recombination in hosts (17) and artificially encouraged recombination in cell culture (30,32) strongly favor homologous recombination Homologous recombination is a type of genetic recombination, a process of physical rearrangement occurring between two strands of DNA. Homologous recombination involves the alignment of similar sequences, a crossover between the aligned DNA strands, and breaking and repair of the and generation of nonredundant hybrid strains, redundant characterization of paired, divergent alleles is inconsistent with a single recombinant genome. The second line of evidence supporting co-infection with independent genomes comes from comparisons of relative co-infectant titers before and after potentially selective events, such as growth in tissue culture. PCR amplification of fiber gene sequences using species B- and E-specific primers was performed on serial dilutions of vaccinated sample 7274 before and after passage of the original ITCF through 2 additional cycles of growth in A549 cells. In this instance, the relative titers of HAdV-4 and HAdV-7, as measured by serial-dilution PCR, changed by 2 orders of magnitude (data not shown). The rapid drift in relative concentrations of PCR targets from paired co-infecting strains strongly suggests that the co-infectants' genomes are replicating independently and thus likely to be physically separate entities. The third line of evidence supporting co-infectant independence comes from whole-genome sequencing efforts. Several molecular methods indicated that vaccinated sample 7151 harbored an HAdV-5/HAdV-21 co-infection (Tables 1 and 2). The genome of the HAdV-5 co-infecting strain was sequenced and assembled into a contiguous sequence (GenBank no. AY601635) consistent with a published HAdV-5 genome (GenBank accession no. AY339865) (40), which suggested no recombination of foreign DNA. However, this effort also generated several orphan sequences that did not fit into the assembled sequence and were subsequently identified as genetically redundant HAdV-21 regions. Further amplification and sequencing of several genetically distant fragments from the same sample using HAdV-21-specific primers yielded [approximately equal to] 2 kb of HAdV-21 sequence. On the basis of the entire genome and partial PCR sequencing analyses, [greater than or equal to] 2 co-infecting HAdV genomes are contained in sample 7151. The fourth line of evidence comes from our attempts to physically separate paired co-infectants by plaque purification. Sample 7151, which contained the HAdV-5/HAdV-21 co-infection, was used initially because it contained relatively equal titers of both co-infectants. Although most of the plaques tested contained HAdV-5, some contained both HAdV-5 and HAdV-21. Although we were unable to identify plaques that contained only HAdV-21, our results demonstrate the physical independence of the co-infecting entities and the functional independence of HAdV-5. Our results also suggest that either the HAdV-21 co-infectant is functionally dependent on HAdV-5 or is effectively outgrown by HAdV-5 to a degree that prevents independent isolation. Similar attempts were made with a few samples that had HAdV-4/HAdV-7 co-infections, but these were generally biased in titer ([10.sup.4] in favor of HAdV-7) and, as expected, yielded only HAdV-7 in >300 plaques tested. The data demonstrated the functional independence of 1 co-infectant (HAdV-7) and physical independence of the co-infecting entities but could not conclusively demonstrate functional independence of the minor co-infectant. Conventional clinical microbiologic methods, including microneutralization and hemagglutination inhibition, are comparative and designed to identify the primary HAdV serotype (or species) in a sample. Secondary infections are masked in these methods by the tests (e.g., microneutralization is reported as the strongest reaction, not the spectrum of reactions across all serotypes). Likewise, direct sequencing (16) may restrict identification to a single strain, particularly if 1 co-infectant is dominant. Restriction enzyme restriction enzyme Protein (more specifically, an endonuclease) produced by bacteria that cleaves DNA at specific sites along its length. Thousands have been found, from many different bacteria; each recognizes a specific nucleotide sequence. analysis methods are capable of resolving HAdV-C dual infections in which both serotypes are present in similar numbers (27). In contrast, when using sensitive molecular methods that can yield measurable signals from secondary (less numerous) co-infectants against the background of stronger signals produced by primary infecting strains, these methods may identify co-infections more than do conventional methods. In the case of respiratory infections, this finding has previously been documented (41). Finally, each of the methods designed to test for multiple species or serotypes showed a higher number of HAdV (and accepted virulent HAdV species and serotypes) in vaccinated persons than in unvaccinated persons. HAdV vaccine was administered routinely to all trainees until supplies were exhausted, at which point adenovirus vaccination was stopped. Since trainees were vaccinated systematically, persons tended to be sampled at times when either all or no recruits were being vaccinated. Therefore, vaccinated samples collected and tested (from 1996 to 1998) are not concurrent with unvaccinated samples (collected from 1998 to 2000). Because of this sampling limitation, we could not confidently correlate HAdV co-infection with breakthrough infections in previously vaccinated persons. Thus, although this study highlights the previously underappreciated phenomenon of adenoviral co-infection, the conclusive examination of its relationship to vaccination must await reintroduction of HAdV vaccine (15). Acknowledgments We thank Gregory C. Gray and Dan Blasiole for critical preceding work, including collection and initial analysis of strains that we reanalyzed, and Beth Metzgar and Valerie de Crecy-Lagard for critically reading the manuscript. Partial support was provided by the Epidemic Outbreak Surveillance Consortium (2) funded by the US Air Force Surgeon General The U.S. Surgeon General is charged with the protection and advancement of health in the United States. Since the 1960s the surgeon general has become a highly visible federal public health official, speaking out against known health risks such as tobacco use, and promoting disease Office, the Modernization modernization Transformation of a society from a rural and agrarian condition to a secular, urban, and industrial one. It is closely linked with industrialization. As societies modernize, the individual becomes increasingly important, gradually replacing the family, Directorate, the Defense Threat Reduction Agency The Defense Threat Reduction Agency (or DTRA) is a combat support agency of the United States Department of Defense (DoD) whose primary function is to analyze potential threats to the United States, both homeland and abroad, and provide contingency plans for all such , and the Office of Naval Research The U.S. Office of Naval Research (ONR), headquartered in Arlington, Virginia (Ballston), is the office within the U.S. Department of the Navy that coordinates, executes, and promotes the science and technology programs of the U.S. . Dr Vora is a research biologist at the Center for Bio/Molecular Science and Engineering, Naval Research Laboratory, Washington, DC. His primary research interest is development of microarray-based molecular diagnostics for human pathogenic microorganisms. References (1.) Rubin BA. Clinical picture and epidemiology of adenovirus infections Adenovirus Infections Definition Adenoviruses are DNA viruses (small infectious agents) that cause upper respiratory tract infections, conjunctivitis, and other infections in humans. Description Adenoviruses were discovered in 1953. . Acta Microbiol Hung. 1993;40:303-23. (2.) Hierholzer JC, Stone YO, Broderson JR. Antigenic relationships among the 47 human adenoviruses determined in reference horse antisera. Arch Virol. 1991;121:179-97. (3.) Wadell G. Molecular epidemiology molecular epidemiology Molecular medicine An evolving field that combines the tools of standard epidemiology–case studies, questionnaires and monitoring of exposure to external factors with the tools of molecular biology–eg, restriction endonucleases, of human adenoviruses. Curr Top Microbiol Immunol. 1984;110:191-220. (4.) Rosen L. A hemagglutination-inhibition technique for typing adenoviruses. Am J Hyg. 1960;71:120-8. (5.) Hierholzer JC. Further subgrouping of the human adenoviruses by differential hemagglutination. J Infect Dis. 1973;128:541-50. (6.) Schmitz H, Wigand R, Heinrich W. Worldwide epidemiology of human adenovirus infections. Am J Epidemiol. 1983;117:455-66. (7.) Brandt CD, Kim HW, Vargosko AJ, Jeffries BC, Arrobio JO, Rindge B, et al. Infections in 18,000 infants and children in a controlled study of respiratory tract respiratory tract n. The air passages from the nose to the pulmonary alveoli, including the pharynx, larynx, trachea, and bronchi. Respiratory tract disease. I. Adenovirus pathogenicity pathogenicity the ability of a pathogenic agent to produce disease in a host. See also virulence. in relation to serologic type and illness syndrome. Am J Epidemiol. 1969;90:484-500. (8.) Fox JP, Hall CE, Cooney MK. The Seattle Virus Watch. VII. Observations of adenovirus infections. Am J Epidemiol. 1977;105:362-86. (9.) Takafuji ET, Gaydos JC, Allen RG, Top FH Jr. Simultaneous administration of live, enteric-coated adenovirus types 4, 7 and 21 vaccines: safety and immunogenicity immunogenicity /im·mu·no·ge·nic·i·ty/ (-je-nis´it-e) the property enabling a substance to provoke an immune response, or the degree to which a substance possesses this property. . J Infect Dis. 1979; 140:48-53. (10.) Van der veen J. The role of adenoviruses in respiratory disease. Am Rev Respir Dis. 1963;88:167-80. (11.) Gooch WM III, Mogabgab WJ. Simultaneous oral administration of live adenovirus types 4 and 7 vaccines: protection and lack of emergence of other types. Arch Environ Health. 1972;25:388-94. (12.) Griffin JP, Greenberg BH. Live and inactivated inactivated rendered inactive; the activity is destroyed. inactivated viruses treated so that they are no longer able to produce evidence of growth or damaging effect on tissue. adenovirus vaccines: clinical evaluation clinical evaluation Medtalk An evaluation of whether a Pt has symptoms of a disease, is responding to treatment, or is having adverse reactions to therapy of efficacy in prevention of acute respiratory disease. Arch Intern intern /in·tern/ (in´tern) a medical graduate serving in a hospital preparatory to being licensed to practice medicine. in·tern or in·terne n. Med. 1970;125:981-6. (13.) Top FH Jr, Dudding BA, Russell PK, Buescher EL. Control of respiratory disease in recruits with types 4 and 7 adenovirus vaccines. Am J Epidemiol. 1971;94:142-6. (14.) Gray GC, Goswami PR, Malasig MD, Hawksworth AW, Trump DH, Ryan MA, et al. Adult adenovirus infections: loss of orphaned vaccines precipitates military respiratory disease epidemics. For the Adenovirus Surveillance Group. Clin Infect Dis. 2000;31:663-70. (15.) Gaydos CA, Gaydos JC. Adenovirus vaccines. In: Plotkin SA, Orenstein WA, Offit PA, editors. Vaccines. Fourth ed. Philadelphia: W.B. Saunders; 2003, p. 863-85. (16.) Blasiole DA, Metzgar D, Daum LT, Ryan MA, Wu J, Wills C, et al. Molecular analysis of adenovirus isolates from vaccinated and unvaccinated young adults. J Clin Microbiol. 2004;42:1686-93. (17.) Kajon AE, Wadell G Sequence analysis of the E3 region and fiber gene of human adenovirus genome type 7h. Virology virology, study of viruses and their role in disease. Many viruses, such as animal RNA viruses and viruses that infect bacteria, or bacteriophages, have become useful laboratory tools in genetic studies and in work on the cellular metabolic control of gene expression . 1996;215:190-6. (18.) Lin B, Vora GJ, Thach D, Walter E, Metzgar D, Tibbetts C, et al. Use of oligonucleotide microarrays for rapid detection and serotyping of acute respiratory disease-associated adenoviruses. J Clin Microbiol. 2004;42:3232-9. (19.) Vabret A, Gouarin S, Joannes M, Barrangcr C, Petitjean J, Corbet S
Corbet is a small village in County Down, Northern Ireland, near Banbridge. In the 2001 Census it had a population of 93 people. It lies within the Banbridge District Council area. , et al. Development of a PCR-and hybridization-based assay (PCR adenovirus consensus) for the detection and the species identification of adenoviruses in respiratory specimens. J Clin Virol. 2004;31:116-22. (20.) Xu W, McDonough MC, Erdman DD. Species-specific identification of human adenoviruses by a multiplex PCR assay. J Clin Microbiol. 2000;38:4114-20. (21.) Crawford-Miksza LK, Nang RN, Schnurr DE Strain variation in adenovirus serotypes 4 and 7a causing acute respiratory disease. J Clin Microbiol. 1999;37:1107-12. (22.) Malasig MD, Goswami PR, Crawford-Miksza LK, Schnurr DP, Gray GC. Simplified microneutralization test for serotyping adenovirus isolates. J Clin Microbiol. 2001;39:2984-6. (23.) Xu W, Erdman DD. Type-specific identification of human adenovirus 3, 7, and 21 by a multiplex PCR assay. J Med Virol. 2001;64:537-42. (24.) Pring-Akerblom P, Trijssenaar FE, Adrian T, Hoyer H. Multiplex polymerase chain reaction for subgenus-specific detection of human adenoviruses in clinical samples. J Med Virol. 1999;58:87-92. (25.) Mei YF, Wadell G. Hemagglutination properties and nucleotide sequence analysis of the fiber gene of adenovirus genome types 11p and 11a. Virology. 1993;194:453-62. (26.) Basler CF, Horwitz MS. Subgroup sub·group n. 1. A distinct group within a group; a subdivision of a group. 2. A subordinate group. 3. Mathematics A group that is a subset of a group. tr.v. B adenovirus type 35 early region 3 mRNAs differ from those of the subgroup C adenoviruses. Virology. 1996;215:165-77. (27.) Fife KH, Ashley R, Shields AF, Salter salt·er n. 1. One that manufactures or sells salt. 2. One that treats meat, fish, or other foods with salt. Noun 1. D, Meyers JD, Corey L. Comparison of neutralization and DNA restriction enzyme methods for typing clinical isolates of human adenovirus. J Clin Microbiol. 1985;22:95-100. (28.) Adhikary AK, Inada T, Banik U, Numaga J, Okabe N. Identification of subgenus subgenus /sub·ge·nus/ (sub´je-nus) a taxonomic category between a genus and a species. sub·ge·nus n. pl. sub·gen·e·ra A taxonomic category ranking between a genus and a species. C adenoviruses by fiber-based multiplex PCR. J Clin Microbiol. 2004;42:670-3. (29.) Hierholzer JC. Adenoviruses in the immunocompromised host An immunocompromised host is a person or lifeform whose immune system has been compromised (either completely or partly) by disease or treatment. . Clin Microbiol Rev. 1992;5:262-74. (30.) Meinschad C, Winnacker EL. Recombination in adenovirus. I. Analysis of recombinant viruses under non-selective conditions. J Gen Virol. 1980;48:219-24. (31.) Boursnell ME, Mautner V. Recombination in adenovirus: crossover sites in intertypic recombinants are located in regions of homology homology (hōmŏl`əjē), in biology, the correspondence between structures of different species that is attributable to their evolutionary descent from a common ancestor. . Virology. 1981 ; 112:198-209. (32.) Sambrook J, Williams J, Sharp PA, Grodzicker T. Physical mapping of temperature-sensitive mutations of adenoviruses. J Mol Biol. 1975;97:369-90. (33.) de Jong De Jong is the most common Dutch surname. Many people bear this name, including many important historical figures. Some of these people are mentioned below. De Jong may mean:
(34.) Kojaoghlanian T, Flomenberg P, Horwitz MS. The impact of adenovirus infection Adenovirus infections most commonly cause illness of the respiratory system; however, depending on the infecting serotype, they may also cause various other illnesses, such as gastroenteritis, conjunctivitis, cystitis, and rash illness. on the immunocompromised host. Rev Med Virol. 2003;13:155-71. (35.) Davison AJ, Benko M, Harrach B. Genetic content and evolution of adenoviruses. J Gen Virol. 2003;84:2895-908. (36.) Stone D, Furthmann A, Sandig V, Lieber A. The complete nucleotide sequence, genome organization, and origin of human adenovirus type 11. Virology. 2003;309:152-65. (37.) Houng HH, Clavio S, Graham K, Kuschner R, Sun W, Russell KL, et al. Emergence of a new human adenovirus type 4 (Ad4) genotype genotype (jēn`ətīp'): see genetics. genotype Genetic makeup of an organism. The genotype determines the hereditary potentials and limitations of an individual. : identification of a novel inverted inverted reverse in position, direction or order. inverted L block a pattern of local filtration anesthesia commonly used in laparotomy in the ox. terminal repeated (ITR See Internet Talk Radio. ) sequence from a majority of Ad4 isolates from US military recruits. J Clin Virol. 2006;35:381-7. (38.) Erdman DD, Xu W, Gerber SI, Gray GC, Schnurr D, Kajon AE, et al. Molecular epidemiology of adenovirus type 7 in the United States United States, officially United States of America, republic (2005 est. pop. 295,734,000), 3,539,227 sq mi (9,166,598 sq km), North America. The United States is the world's third largest country in population and the fourth largest country in area. , 1966-2000. Emerg Infect Dis. 2002;8:269-77. (39.) Li Q, Wadell G. Genetic variability Introduction Genetic Variability
(40.) Sugarman BJ, Hutchins BM, McAllister DL, Lu F, Thomas BK. The complete nucleic acid nucleic acid, any of a group of organic substances found in the chromosomes of living cells and viruses that play a central role in the storage and replication of hereditary information and in the expression of this information through protein synthesis. sequence of the adenovirus type 5 reference material (ARM) genome. Bioprocessing Journal. 2003;2:27-32. (41.) Mitchell S Mitchell, city (1990 pop. 13,798), seat of Davison co., SE S.Dak.; inc. 1881. Mitchell is a trade, distribution, and shipping center for a dairy and livestock area. , O'Neill HJ, Ong GM, Christie S, Duprex P, Wyatt DE, et al. Clinical assessment of a generic DNA amplification DNA amplification Molecular diagnostics Any method used to ↑ the copy number of a sequence of DNA. See Cycling probe technology, Gap LCR–gap ligase chain reaction, Gene amplification, NASBA–nucleic acid sequence-based amplification, PCR, assay for the identification of respiratory adenovirus infections. J Clin Virol. 2003;26:331-8. Address for correspondence: David Metzgar, Naval Health Research Center, PO Box 85122, San Diego San Diego (săn dēā`gō), city (1990 pop. 1,110,549), seat of San Diego co., S Calif., on San Diego Bay; inc. 1850. San Diego includes the unincorporated communities of La Jolla and Spring Valley. Coronado is across the bay. , CA 92186-5122, USA; email: metzgar@nhrc.navy.mil (2) The members of the Epidemic Outbreak Surveillance Consortium are Peter F. Demitry, Theresa Lynn Difato, Robb K. Rowley, Clark Tibbetts, Eric H. Hanson, Rosana R. Holliday, Curtis White, David A. Stenger, Donald Seto, Elizabeth A. Walter, Jerry Diao, Brian K. Agan, Kevin Russell Kevin Richard Russell (* 12 January 1964 in Hamburg is a German musician and belongs to the three founding members of the German rock band Böhse Onkelz. Since 1980 until the breakup of the band in the year 2005 he was their singer. , David Metzgar, Gary J. Vora, Baochuan Lin, Dzung Thach, Jing jing (jing) [Chinese] one of the basic substances that according to traditional Chinese medicine pervade the body, usually translated as "essence"; the body reserves or constitutional makeup, replenished by food and rest, that supports Su, Chris Olsen, Dong Xia, John Gomez, John McGraw Noun 1. John McGraw - United States baseball player and manager (1873-1934) John Joseph McGraw, McGraw , Linda Canas, Margaret Jesse, Mi Ha Yuen, Robert Crawford Robert Crawford (born 4th July 1886, died ca. 1950) was a footballer who played for Liverpool Football Club during the early part of the 20th century. Life and playing career , Sue A. Worthy, Sue Ditty dit·ty n. pl. dit·ties A simple song. [Middle English dite, a literary composition, from Old French dite, from Latin dict , John McGraw, Michael Jenkins, Zheng Wang, Cheryl J. James, Kathy Ward, Kenya Grant, and Kindra Nix. Gary J. Vora, * ([dagger], 1) Baochuan Lin, * ([dagger] 1) Kevin Gratwick, ([double dagger double dagger n. A reference mark (  ) used in printing and writing. Also called diesis.Noun 1. ]) Carolyn Meador, ([section]) Christian Hansen Christian Marius Hansen (born September 24, 1891 - died June 13, 1961) was a Danish gymnast who competed in the 1908 Summer Olympics and in the 1912 Summer Olympics. He was part of the Danish team, which finished fourth in the gymnastics team event in 1908. , ([double dagger]) Clark Tibbetts, ([dagger]) David A. Stenger, * ([dagger]) Marina Irvine, ([double dagger]) Donald Seto, ([dagger] [paragraph]) Anjan Purkayastha, ([dagger] [paragraph]) Nikki E. Freed, ([double dagger]) Marylou GL Gibson, (#) Kevin Russell, ([dagger] [double dagger]) and David Metzgar ([dagger] [double dagger]) (1) These authors contributed equally to this article. * Naval Research Laboratory, Washington, DC, USA; ([dagger]) Epidemic Outbreak Surveillance Consortium, Falls Church, Virginia Falls Church is an independent city in Virginia, United States. The population was 10,377 at the 2000 census. This city is a part of the Washington Metropolitan Area. A much larger number of people reside in Greater Falls Church , USA; ([double dagger]) Naval Health Research Center, San Diego, California “San Diego” redirects here. For other uses, see San Diego (disambiguation). San Diego is a coastal Southern California city located in the southwestern corner of the continental United States. As of 2006, the city has a population of 1,256,951. , USA; ([section]) Nova Research Inc., Alexandria, Virginia Alexandria is an independent city in the Commonwealth of Virginia. As of the 2000 census, the city had a total population of 128,284. Located along the Western bank of the Potomac River, Alexandria is approximately 6 miles (9.6 kilometers) south of downtown Washington, DC. , USA; ([paragraph]) George Mason University Named after American revolutionary, patriot and founding father George Mason, the university was founded as a branch of the University of Virginia in 1957 and became an independent institution in 1972. , Manassas, Virginia “Manassas” redirects here. For other uses, see Manassas (disambiguation). Manassas is an independent city located in the Commonwealth of Virginia. The population was 35,135 at the 2000 census. , USA; and (#) Virapur, LLC (Logical Link Control) See "LANs" under data link protocol. LLC - Logical Link Control , San Diego, California, USA
Table 1. Naval Health Research Center data for molecular detection of
adenoviral co-infections in vaccinated and unvaccinated patients with
febrile respiratory illness *
Microneu-
Vaccination tralization
Original designation ([dagger]) date ([double dagger])
7151.AV5.V.98.FJ 5 Nov 1997 4
7137.AV4.V.97.FJ 1 Dec 1997 4
7274.AV4.V.98.FJ 11 Feb 1998 4
7307.AV5.V.98.FJ 9 Feb 1998 4
7333.AV4.V.98.FJ 25 Mar 1998 4
4185.AV4.V.97.FLW 24 Mar 1997 4
4476.AV4.V.97.FLW 24 Oct 1997 4
79.AV4.V.96.GL 7 Oct 1996 4
141.AV7.V.96.GL 12 Nov 1996 7
275.AV4.V.97.GL 31 Jan 1997 4
1212.AV7.V.97.GL 29 Sep 1997 7
1108.AV7.V..97.GL 8 Oct 1997 7
1122.AV7.V.97.GL 8 Oct 1997 7
1150.AV7.V.97.GL 8 Oct 1997 7
1152.AV7.V.97.GL 8 Oct 1997 7
1186.AV7.V.97.GL 8 Oct 1997 7
1251.AV7.V.97.GL 8 Oct 1997 7
1275.AV7.V.97.GL 8 Oct 1997 7
1302.AV7.V.97.GL 8 Oct 1997 7
1649.AV7.V.98.GL 13 Jan 1998 7
1856.AV5.V.98.GL 25 Mar 1998 4
60406.AV7.99.FB 7
60673.AV4.00.FB 4
60691.AV4.00.FB 4
60697.AV4.00.FB 4
60708.AV4.00.FB 4
60716.AV4.00.FB 4
CHPPM2.AV4.00.FB
CHPPM9.AV4.00.FB 4
CHPPM13.AV4.00.FB
CHPPM29.AV4.00.FB 4
CHPPM44.AV4.00.FB 4
7372.AV5.98.FJ 4
40098.AV4.98.FJ 4
40160.AV4.98.FJ 4
40183.AV4.98.FJ 4
40781.AV4.99.FJ 4
40844.AV4.99.FJ 4
41059.AV4.99.FJ 4
10060.AV4.98.GL
10190.AV4.98.GL 4
10206.AV4.98.GL 4
10213.AV4.98.GL 4
10257.AV4.98.GL 4
10258.AV4.98.GL 4
10756.AV4.00.GL 4
50108.AV4.00.LAC
20044.AV4.98.MCRD 4
20139.AV4.98.MCRD
20142.AV4.98.MCRD
20143.AV4.98.MCRD
20145.AV4.98.MCRD
Species-
Multiplex specific PCR
Original designation ([dagger]) PCR (B, C, E)
7151.AV5.V.98.FJ B, C B, C, E
7137.AV4.V.97.FJ E B, E
7274.AV4.V.98.FJ E, B E, B
7307.AV5.V.98.FJ C, B B, C, E
7333.AV4.V.98.FJ E E, B#
4185.AV4.V.97.FLW E B, E
4476.AV4.V.97.FLW E B, E
79.AV4.V.96.GL E E
141.AV7.V.96.GL B B
275.AV4.V.97.GL E E
1212.AV7.V.97.GL B B, E
1108.AV7.V..97.GL E, B B, E
1122.AV7.V.97.GL B B
1150.AV7.V.97.GL B B, E
1152.AV7.V.97.GL B B
1186.AV7.V.97.GL B B, E
1251.AV7.V.97.GL B B
1275.AV7.V.97.GL B B, E
1302.AV7.V.97.GL B B, E
1649.AV7.V.98.GL B B
1856.AV5.V.98.GL C B, C, E
60406.AV7.99.FB B B
60673.AV4.00.FB E E
60691.AV4.00.FB E E, B#
60697.AV4.00.FB E E
60708.AV4.00.FB E E
60716.AV4.00.FB E E
CHPPM2.AV4.00.FB E E, B#
CHPPM9.AV4.00.FB E E, B#
CHPPM13.AV4.00.FB E E, B#
CHPPM29.AV4.00.FB E E
CHPPM44.AV4.00.FB E E
7372.AV5.98.FJ C B, C, E
40098.AV4.98.FJ E E
40160.AV4.98.FJ E E, B#
40183.AV4.98.FJ E E
40781.AV4.99.FJ E E
40844.AV4.99.FJ E E
41059.AV4.99.FJ E E
10060.AV4.98.GL E E
10190.AV4.98.GL E E, B#
10206.AV4.98.GL E E
10213.AV4.98.GL E E
10257.AV4.98.GL E E
10258.AV4.98.GL E E
10756.AV4.00.GL E E
50108.AV4.00.LAC E B, E
20044.AV4.98.MCRD E B, E
20139.AV4.98.MCRD E E
20142.AV4.98.MCRD E E
20143.AV4.98.MCRD E E, B#
20145.AV4.98.MCRD E E
GenBank
accession
Original designation ([dagger]) Sequencing ([section]) no.
7151.AV5.V.98.FJ 5, 21
7137.AV4.V.97.FJ 4 variant AY337237
7274.AV4.V.98.FJ 4 vaccine ([DELTA] = 2) AF065062
7307.AV5.V.98.FJ 5
7333.AV4.V.98.FJ 4 variant AY337242
4185.AV4.V.97.FLW 4 variant, 7h AY337252
4476.AV4.V.97.FLW 4 variant AY337249
79.AV4.V.96.GL 4 vaccine ([DELTA] = 3) AF065062
141.AV7.V.96.GL 7d2 (prototype) AY337258
275.AV4.V.97.GL 4 vaccine ([DELTA] = 3) AY337239
1212.AV7.V.97.GL 7d2 ([DELTA] = 2) AY337255
1108.AV7.V..97.GL 7 vaccine ([DELTA] = 0) AF065067
1122.AV7.V.97.GL 7d2 ([DELTA] = 2) AF321311
1150.AV7.V.97.GL 7 vaccine ([DELTA] = 2) AY337254
1152.AV7.V.97.GL 7 vaccine ([DELTA] = 1) AY337253
1186.AV7.V.97.GL 7d2 ([DELTA] = 2) AF321311
1251.AV7.V.97.GL 7d2 ([DELTA] = 2) AF321311
1275.AV7.V.97.GL 7 vaccine ([DELTA] = 1) AY337257
1302.AV7.V.97.GL 7 vaccine ([DELTA] = 2) AY337256
1649.AV7.V.98.GL 7d2 ([DELTA] = 2) AF321311
1856.AV5.V.98.GL 5, 7h
60406.AV7.99.FB 7 vaccine ([DELTA] = 2) AY337256
60673.AV4.00.FB 4 variant AY337237
60691.AV4.00.FB 4 variant AY337238
60697.AV4.00.FB 4 variant AY337246
60708.AV4.00.FB 4 variant AY337237
60716.AV4.00.FB 4 variant AY337247
CHPPM2.AV4.00.FB 4 variant AY337237
CHPPM9.AV4.00.FB 4 variant AY337237
CHPPM13.AV4.00.FB 4 variant AY337237
CHPPM29.AV4.00.FB 4 variant AY337237
CHPPM44.AV4.00.FB 4 variant AY337237
7372.AV5.98.FJ 5, 7h
40098.AV4.98.FJ 4 variant AY337241
40160.AV4.98.FJ 4 variant AY337237
40183.AV4.98.FJ 4 variant AY337237
40781.AV4.99.FJ 4 variant AY337238
40844.AV4.99.FJ 4 variant AY337237
41059.AV4.99.FJ 4 variant AY337237
10060.AV4.98.GL 4 variant AY337237
10190.AV4.98.GL 4 variant AY337237
10206.AV4.98.GL 4 variant AY337244
10213.AV4.98.GL 4 variant AY337240
10257.AV4.98.GL 4 variant AY337237
10258.AV4.98.GL 4 variant AY337237
10756.AV4.00.GL 4 variant AY337243
50108.AV4.00.LAC 4 variant AY337251
20044.AV4.98.MCRD 4 variant AY337248
20139.AV4.98.MCRD 4 variant AY337237
20142.AV4.98.MCRD 4 variant AY337250
20143.AV4.98.MCRD 4 variant AY337237
20145.AV4.98.MCRD 4 variant AY337245
* PCR, polymerase cnain reaction. Letters or numbers in boldface
indicate weak positives.
([dagger]) Acquisition number, serotype, isolation year, and isolation
location.
([double dagger]) Results are listed as serotypes. Species B1 includes
serotypes 3, 7, 16, 21; species C includes serotypes 1, 2, 5, 6;
and species E includes serotype 4.
([section]) Variant/vaccine grouping based on the hexon gene sequence
defined by Blasiole et al. (16). [DELTA] = # reflects number of base
substitutions from vaccine strain in 1,490 by of the hexon sequence
(16). The 7h designation is based on that of Blasiole et al. (16).
The 7h designation based on fiber gene sequence is as defined by Kajon
and Wadell (17).
Note: Figures in bold indicated with #.
Table 2. Naval Research Laboratory data for molecular detection of
adenoviral co-infections in vaccinated and unvaccinated patients
with febrile respiratory illness *
Original designation Microarray
([dagger]) Vaccination date ([double dagger])
7151.AV5.V.98.FJ 5 Nov 1997 C, 21
7137.AV4.V.97.FJ 1 Dec 1997 4, C, B2
7274.AV4.V.98.FJ 11 Feb 1998 4, 21, C, B2
7307.AV5.V.98.FJ 9 Feb 1998 C, 21
7333.AV4.V.98.FJ 25 Mar 1998 4, C, B2
4185.AV4.V.97.FLW 24 Mar 1997 4, C, B2
4476.AV4.V.97.FLW 24 Oct 1997 4, C, B2
79.AV4.V.96.GL 7 Oct 1996 4, C, 7
141.AV7.V.96.GL 12 Nov 1996 7, 4, 3#
275.AV4.V.97.GL 31 Jan 1997 4, C, 7
1212.AV7.V.97.GL 29 Sep 1997 7, 4, 3#
1108.AV7.V..97.GL 8 Oct 1997 7, 4, C, 3#
1122.AV7.V.97.GL 8 Oct 1997 7, C, 3#
1150.AV7.V.97.GL 8 Oct 1997 7, 4, 3#
1152.AV7.V.97.GL 8 Oct 1997 7, 4, 3#
1186.AV7.V.97.GL 8Oct 1997 7, 4
1251.AV7.V.97.GL 8Oct 1997 7, 4, 3#
1275.AV7.V.97.GL 8 Oct 1997 7, 4, 3#
1302.AV7.V.97.GL 8Oct 1997 7, 4, 3#
1649.AV7.V.98.GL 13 Jan 1998 7, 3, 4
1856.AV5.V.98.GL 25 Mar 1998 C, 7#
60406.AV7.99.FB 7
60673.AV4.00.FB 4, C
60691.AV4.00.FB 4, C
60697.AV4.00.FB 4, C
60708.AV4.00.FB 4, C
60716.AV4.00.FB 4, C
CHPPM2.AV4.00.FB 4, C
CHPPM9.AV4.00.FB 4, C
CHPPM13.AV4.00.FB 4, C
CHPPM29.AV4.00.FB 4, C
CHPPM44.AV4.00.FB 4, C
7372.AV5.98.FJ C, 7#
40098.AV4.98.FJ 4
40160.AV4.98.FJ 4
40183.AV4.98.FJ 4
40781.AV4.99.FJ 4, C
40844.AV4.99.FJ 4, C
41059.AV4.99.FJ 4, C
10060.AV4.98.GL 4, C, B2
10190.AV4.98.GL 4
10206.AV4.98.GL 4, C, B2
10213.AV4.98.GL 4, C, B2#
10257.AV4.98.GL 4, B2
10258.AV4.98.GL 4
10756.AV4.00.GL 4
50108.AV4.00.LAC 4, B2
20044.AV4.98.MCRD 4, C, 7, 3#
20139.AV4.98.MCRD 4
20142.AV4.98.MCRD 4
20143.AV4.98.MCRD 4, C, B2
20145.AV4.98.MCRD 4, C, B2
PCR determination
([double dagger])
Original designation Adenovirus
([dagger]) Consensus kit Positive Negative
7151.AV5.V.98.FJ C, B1 5, 21
7137.AV4.V.97.FJ E 4, 1 B2
7274.AV4.V.98.FJ E, B1, B2 4, 21, B2 C
7307.AV5.V.98.FJ C C 21
7333.AV4.V.98.FJ E 4, 1, 5, B2
4185.AV4.V.97.FLW E, 82, F, B1 4, B2 C
4476.AV4.V.97.FLW E, B2, F, B1 4, 5, B2
79.AV4.V.96.GL E 4, C, B2 7
141.AV7.V.96.GL B1, B2, E 7, 4, B2 3
275.AV4.V.97.GL E, B2, F, B1 4, C, B2 7
1212.AV7.V.97.GL B1, E, F 7, 4, 3, F
1108.AV7.V..97.GL B1, E, F 7, 4, C 3
1122.AV7.V.97.GL B1 7, C 3
1150.AV7.V.97.GL B1, E, F 7, 3, F 4
1152.AV7.V.97.GL 131 7, 4 3
1186.AV7.V.97.GL 131, E, F 7 4
1251.AV7.V.97.GL 131, E, F 7 4, 3
1275.AV7.V.97.GL B1, E 7, 4, 3
1302.AV7.V.97.GL B1, E, F 7, 4 3
1649.AV7.V.98.GL B1 7, 3 4
1856.AV5.V.98.GL C C 7
60406.AV7.99.FB B 1 7
60673.AV4.00.FB E 4 C
60691.AV4.00.FB E 4 C
60697.AV4.00.FB E 4, 1
60708.AV4.00.FB E 4 C
60716.AV4.00.FB E 4 C
CHPPM2.AV4.00.FB E 4 C
CHPPM9.AV4.00.FB E 4 C
CHPPM13.AV4.00.FB E 4 C
CHPPM29.AV4.00.FB E 4 C
CHPPM44.AV4.00.FB E 4 C
7372.AV5.98.FJ C C 7
40098.AV4.98.FJ E, F 4, F
40160.AV4.98.FJ E 4
40183.AV4.98.FJ E 4
40781.AV4.99.FJ E, B2 4, B2 C
40844.AV4.99.FJ E, B2 4, B2 C
41059.AV4.99.FJ E, B2, F 4, C, B2, F
10060.AV4.98.GL E, B2 4, B2 C
10190.AV4.98.GL E 4
10206.AV4.98.GL E, B2 4, B2 C
10213.AV4.98.GL E, B2, F 4, B2
10257.AV4.98.GL E 4, B2
10258.AV4.98.GL E 4
10756.AV4.00.GL E 4
50108.AV4.00.LAC E 4, B2
20044.AV4.98.MCRD E 4, 1, B2 73
20139.AV4.98.MCRD E 4
20142.AV4.98.MCRD E 4
20143.AV4.98.MCRD E, B2, F 4, C, B2, F
20145.AV4.98.MCRD E, B2, F 4, B2
* PCR, polymerase chain reaction. Species and serotype are listed in
order of predominance. Letters or numbers in boldface indicate weak
positives.
([dagger]) Acquisition number, serotype, isolation year, and isolation
location.
([double dagger]) Results are listed as serotypes or species. Species
B1 includes serotypes 3, 7, 16, 21; species C includes serotypes
1, 2, 5, 6; and species E includes serotype 4.
Note: Figures in bold indicated with #.
Table 3. Human adenovirus load detected with molecular identification
methods *
No. samples with X
co-infectant strains
Method Status X = 1 X = 2 X = 3 X = 4
Microarray Vaccinated 0 4 15 2
Unvaccinated 9 16 5 1
Adenovirus Consensus kit Vaccinated 8 2 8 3
Unvaccinated 22 5 4 0
Multiplex PCR Vaccinated 17 4 0 0
Unvaccinated 31 0 0 0
Monoplex PCR ([dagger]) Vaccinated 7 11 3 0
Unvaccinated 21 9 1 0
* PCR, polymerase chain reaction.
([dagger]) Species-specific PCR from Table 1, Naval Health
Research Center data.
Table 4. Human adenovirus (HAdV) species and serotype-specific primers
Name Sequence Target gene
Primer 1 CTT GGT CTA CGA CCA GAC GG
Primer 3 GTT TGC TCA TGA ACA TGG CCA GAT CGC AC Species B2 E3
F30 CTT CAA CCC TGT CTA CCC TAT GAA
F969 TTC TCT AAT GTA GTA AAA GG HAdV11 fiber
HsgF1 ATT TCT ATT CCT TCG CG
HsgF2 TCA GGC TTG GTA CGG CC Species F hexon
HsgC1 ACC TTT GAC TCT TCT GT
HsgC2 TCC TTG TAT TTA GTA TC Species C hexon
Ad3F GGT AGA GAT GCT GTT GCA GGA
Ad3R CCC ATC CAT TAG TGT CAT CGG T HAdV3 hexon
Ad7F GGA AAG ACA TTA CTG CAG ACA
Ad7R AAT TTC AGG CGA AAA AGC GTC A HAdV7 hexon
Ad21F GAA ATT ACA GAC GGC GAA GCC
Ad21R AAC CTG CTG GTT TTG CGG TTG HAdV21 hexon
Ad4F5 GTT GCT AAC TAC GAT CCA GAT ATT G
Ad4R4 CCT GGT AAG TGT CTG TCA ATC C HAdV4 hexon
Ad7F-F ACA ACT GCC TAT CCT TTC AAT G
Ad7F-R GAC CAA GTT ACA CGA ATA CAA TAT G HAdV7 fiber
Ad5 E1A-F1 CCT AAA ATG GCG CCT GCT ATC CTG
Ad5 E1A-R1 GCG ACG CCC ACC AAC TCT CAC HAdV5 E1A
Ad5 E1A-F2 GAG CCT TGG GTC CGG TTT CTA TG
Ad5 E1A-R2 CCA TTT TAG GAC GGC GGG TAG HAdV5 E1A
Ad5 hexon-F1 GAC GGA GCC AGC ATT AAG TTT GAT
Ad5 hexon-R1 GTT GGC GGG TAT AGG GTA GAG CAT HAdV5 hexon
Ad5 fiber-F1 TAT TCA GCA TCA CCT CCT TTC C
Ad5 fiber-R1 AAG CTA TGT GGT GGT GGG GC HAdV5 fiber
AdA1 GCT GAA GAA MCW GAA GAA AAT GA
AdA2 CRT TTG GTC TAG GGT AAG CAC Species A fiber
AdB1 TST ACC CYT ATG AAG ATG AAA GC
AdB2 GGA TAA GCT GTA GTR CTK GGC AT Species B fiber
AdC1 TAT TCA GCA TCA CCT CCT TTC C
AdC2 AAG CTA TGT GGT GGT GGG GC Species C fiber
AdD1 GAT GTC AAA TTC CTG GTC CAC
AdD2 TAC CCG TGC TGG TGT AAA AAT C Species D fiber
AdE1 TCC CTA CGA TGC AGA CAA CG
AdE2 AGT GCC ATC TAT GCT ATC TCC Species E fiber
AdF1 ACT TAA TGC TGA CAC GGG CAC
AdF2 TAA TGT TTG TGT TAC TCC GCT C Species F fiber
Name Reference
Primer 1
Primer 3 (26)
F30
F969 (25)
HsgF1
HsgF2 (24)
HsgC1
HsgC2 (24)
Ad3F
Ad3R (23)
Ad7F
Ad7R (23)
Ad21F
Ad21R (23)
Ad4F5
Ad4R4 This study
Ad7F-F
Ad7F-R This study
Ad5 E1A-F1
Ad5 E1A-R1 This study
Ad5 E1A-F2
Ad5 E1A-R2 This study
Ad5 hexon-F1
Ad5 hexon-R1 This study
Ad5 fiber-F1
Ad5 fiber-R1 This study
AdA1
AdA2 (20)
AdB1
AdB2 (20)
AdC1
AdC2 (20)
AdD1
AdD2 (20)
AdE1
AdE2 (20)
AdF1
AdF2 (20)
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