Pneumocystis jirovecii in general population.The possible presence of Pneumocystis Pneumocystis /Pneu·mo·cys·tis/ (-sis´tis) a genus of yeastlike fungi. P. cari´nii is the causative agent of interstitial plasma cell pneumonia. pneu·mo·cys·tis n. among healthy adults was examined by detecting Pneumocystis jirovecii--specific 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. in prospectively obtained oropharyngeal oropharyngeal /oro·pha·ryn·ge·al/ (-fah-rin´je-al) 1. pertaining to the mouth and pharynx. 2. pertaining to the oropharynx. wash samples from 50 persons without underlying lung disease or immunosuppression immunosuppression Suppression of immunity with drugs, usually to prevent rejection of an organ transplant. Its aim is to allow the recipient to accept the organ permanently with no unpleasant side effects. . Pneumocystis carriage, defined by detecting Pneumocystis DNA by nested polymerase chain reaction Nested polymerase chain reaction is a modification of polymerase chain reaction intended to reduce the contaminations in products due to the amplification of unexpected primer binding sites. in 2 independent analyses plus successful mitochondrial mitochondrial pertaining to mitochondria. mitochondrial RNAs a unique set of tRNAs, mRNAs, rRNAs, transcribed from mitochondrial DNA by a mitochondrial-specific RNA polymerase, that account for about 4% of the total cell RNA that large subunit ribosomal RNA typing by direct sequencing, was found in 20% of cases. All carriers were asymptomatic, anti-HIV negative, and had normal total lymphocyte and CD4+ cell counts. A second sample obtained in the 6-month follow-up was positive in 2 of 9 available carriers. Genotype analysis showed different polymorphisms; 85A/248C (40%) and 85C/248C (30%) were most frequently observed. This study provides the first evidence that P. jirovecii DNA can be frequently detected in the respiratory tract of immunocompetent im·mu·no·com·pe·tent adj. Having the normal bodily capacity to develop an immune response following exposure to an antigen. im adults, which agrees with the hypothesis that the general population could be a reservoir and source of this infection. ********** Pneumocystis jirovecii (formerly known as Pneumocystis carinii f. sp. hominis) (1) is the causative agent of Pneumocystis pneumonia (PCP PCP abbr. 1. phencyclidine 2. primary care physician Pneumocystis carinii pneumonia (PCP) ), one of the most frequent and severe opportunistic infections 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 (2). Pneumocystis organisms represent a large group of species of atypical fungi with universal distribution and pulmonary tropism tropism (trōp`ĭzəm), involuntary response of an organism, or part of an organism, involving orientation toward (positive tropism) or away from (negative tropism) one or more external stimuli. , and each species has a strong specificity for a given mammalian host species (3,4). Despite the advances made in understanding human Pneumocystis infection, many aspects about its epidemiology and natural history remain unclear. Serologic studies have shown that specific antibodies to the pathogen can be detected in most children early in life (5-7), which indicates frequent exposure to this organism. Based on this finding, disease in immunocompromised persons has long been thought to result from reactivation of latent infection acquired in childhood. However, animal and human studies have shown that elimination of Pneumocystis often occurs after infection (8-9), which implies that the persistence of latent organisms is limited. Alternatively, the possibility that Pneumocystis can be transmitted from person to person has been raised after the reports of cluster outbreaks of PCP among solid-organ transplant and oncology patients (10,11). Evidence supporting the active or de novo airborne acquisition of the organism from human sources has accumulated in the last few years, including evidence for different Pneumocystis genotypes in different episodes of PCP in the same patient (12,13). Also, Pneumocystis DNA was detected in the upper respiratory tract of healthy participants after close contact with patients with PCP (14-16) and in air samples from the rooms of PCP patients (17,18). Pneumocystis has also been found in immunosuppressed Immunosuppressed A state in which the immune system is suppressed by medications during the treatment of other disorders, like cancer, or following an organ transplantation. Mentioned in: Fifth Disease patients without PCP (19); these situations have been described as Pneumocystis colonization or carriage. PCP patients, immunodeficient carriers, or transiently parasitized immunocompetent persons have been hypothesized to play a role as sources of Pneumocystis infection (4). Although some earlier studies failed to detect the organism in postmortem lung samples or bronchoalveolar samples from immunocompetent adults (20,21), a recent report indicates that Pneumocystis DNA can be frequently detected in healthy infants (22). The ability to detect Pneumocystis in normal, healthy persons is due to the development of more sensitive methods. Pneumocystis can now be detected in respiratory samples obtained by noninvasive methods using immunofluorescence staining and 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) ) (23,24). By using these methods, Pneumocystis carriage was found in 10% to 40% of immunocompetent patients with different chronic lung diseases (25,26). From an epidemiologic point of view, this high prevalence is difficult to determine if PCP or colonized Colonized This occurs when a microorganism is found on or in a person without causing a disease. Mentioned in: Isolation immunosuppressed patients and their close contacts are the only sources of infection, since the persistence of latent organism in lung appears to be time-limited (8,9). We tested the hypothesis that in a normal community environment healthy adults can be transiently colonized by Pneumocystis, and these persons play a role in the persistence of the organism in the human ecosystem. Identifying Pneumocystis sources is essential to developing proper measures to prevent a disease that still causes substantial illness and death among immunosuppressed patients. This study attempts to determinate whether P. jirovecii can be detected in the general normal, healthy population. Methods Study Population This prospective study included persons who 1) had not been exposed to patients in a hospital environment within the year before the study or 2) had not been diagnosed with or were not suspected to have chronic lung disease, neoplasm neoplasm or tumor, tissue composed of cells that grow in an abnormal way. Normal tissue is growth-limited, i.e., cell reproduction is equal to cell death. , or immunosuppression of any cause. The first 50 persons evaluated in the Occupational Health Service of the Virgen del Rocio University Hospital from February to July 2003 who had not been excluded by the above criteria were enrolled in this study. The mean age of persons in this study group was 33.9 [+ or -] 9.45 years. Nineteen (31.6%) were male. Distribution according to professional standing was 28 (56%) newly employed physician residents, 13 (26%) university or common services staff members, and 9 (18%) administrative staff. Each participant underwent a clinical-epidemiologic examination, and oropharyngeal samples were collected for analysis in the Occupational Health Service, a building located outside the hospital environment. Demographic variables, underlying medical conditions, habits, and antimicrobial therapy were recorded by using a standardized form. Informed consent was obtained from participants. The study protocol was designed and performed according to the Helsinki Declaration and was approved by the ethics committee, Virgen del Rocio University Hospital, Seville, Spain. For all Pneumocystis carriers, a complete clinical and biologic evaluation was performed, including physical examination, chest x-ray, conventional blood work, anti-HIV serologic examination, and peripheral blood lymphocyte subsets analyses. Volunteers who were designated P. jirovecii carriers were reexamined after 6 months, when oropharyngeal samples were again obtained. Case Definition A Pneumocystis carrier was defined as a person who met all of the following conditions: 1) no clinical history of PCR 2) respiratory specimen with detectable P. jirovecii DNA by nested PCR in 2 independent analyses, and 3) successful mitochondrial large subunit ribosomal RNA (mtLSU-rRNA) typing of the respiratory specimen by direct sequencing at least once. Persons who did not meet these criteria were considered Pneumocystis-negative. Sampling and Detecting P. jirovecii Oropharyngeal wash samples were obtained by gargling Gargling is a common method of cleansing the throat, especially if one has a sore throat or upper-respiratory virus or infection. The physical act of gargling usually requires that one tilts the head back, allowing a mouthful of liquid to sit in the upper throat. with 10 mL of sterile physiologic serum (0.9% NaCl) for a period of 1 min. Samples were centrifuged at 2,900 x g for 5 min and kept frozen at -20[degrees]C until DNA was extracted. After digestion with proteinase proteinase /pro·tein·ase/ (pro´ten-as?) endopeptidase. pro·tein·ase n. A protease that begins the hydrolytic breakdown of proteins usually by splitting them into polypeptide chains. K at 56[degrees]C for 2 h, DNA from 2 aliquots of each oropharyngeal wash sample was extracted on 2 days by using a commercial kit from Qiagen (Hilden, Germany). Sham extractions, carried out in parallel with the processing of samples, were also included to control for contamination in the DNA extraction step. The purified DNA was used as a template to amplify the region containing mtLSU-rRNA by nested PCR, as described elsewhere (27,28). The sensitivity of this nested PCR assay is 1 organism/[micro]L. Briefly, in the first amplification round, the external primers pAZ102-E (5'-GAT GGC GGC Girl Guides of Canada GGC Greenwood Genetic Center (South Carolina) GGC Gwasanaeth Gwaed Cymru (Welsh Blood Service) GGC Generalized Goppa Code GGC Grosvenor Gallery Company TGT TGT Target TGT Ticket Granting Ticket (Windows 2000 Kerberos security) TGT Target Corp (stock symbol) TGT Turbine Gas Temperature TGT TDRSS Ground Terminal TGT Tank Gunnery Trainer TGT Target Tracker TTC TTC Trying To Conceive TTC Toronto Transit Commission TTC Trans Texas Corridor TTC Toutes Taxes Comprises (French) TTC Trident Technical College (North Charleston, SC) TTC Temporary Traffic Control CAA Caa See CCC. GCC GCC: see Gulf Cooperation Council. (compiler, programming) GCC - The GNU Compiler Collection, which currently contains front ends for C, C++, Objective-C, Fortran, Java, and Ada, as well as libraries for these languages (libstdc++, libgcj, etc). CA-3') and pAZ102-H (5'-GTG TAC 1. TAC - Translator Assembler-Compiler. For Philco 2000. 2. TAC - Terminal Access Controller. GTT GTT, n See test, glucose tolerance. GTT Glucose tolerance test, see there GCA GCA, ground-controlled approach: see instrument-landing system. AAG AAG Association of American Geographers (Washington, DC) AAG Assistant Attorney General AAG Asociación Argentina de Golf AAG Anti-Aircraft Gun AAG Assistant Adjutant General AAG Australian Association of Gerontology TAC TC-3') were used. This amplification yields a 346-base pair (bp) fragment. The second round of amplification used the primers pAZ102-X (5'-GTG AAA AAA: see American Automobile Association. (Triple A) A common single-cell battery used in a myriad of electronic devices of all variety. Like its double A (AA) cousin, it provides 1.5 volts of DC power. When used in series, the voltage is multiplied. TAC AAA TCG (Trusted Computing Group, Beaverton, OR, www.trustedcomputinggroup.org) The successor to the Trusted Computer Platform Alliance (TCPA), announced in 2003 by founding members AMD, HP, IBM, Intel and Microsoft. GAC GAC Great American Country GAC Global Assembly Cache (Microsoft .NET) GAC Global Assembly Cache GAC Granular Activated Carbon GAC Gustavus Adolphus College (St. TAG G-3") and pAZ102-Y (5'-TCA CTT CTT Correios (Portuguese Postal Service) CTT Certified Technical Trainer CTT Charity Technology Trust CTT Cholesterol Treatment Trialists' (collaboration) CTT Common Task Training AAT Alpha-1-antitrypsin (AAT) A blood component that breaks down infection-fighting enzymes such as elastase. Mentioned in: Chronic Obstructive Lung Disease ATT ATT ammonia tolerance test. AAT TGG TGG The Great Gatsby (novel F. Scott Fitzgerald; movie) TGG Kuala Terengganu, Malaysia - Sultan Mahmood (Airport Code) TGG Temporary Geographic Grid TGG Third Generation Gyro TGG Triple Graph Grammar GGA GGA Generalized Gradient Approximation GGA Good Game All ggA Geschützte Geographische Angabe (German: Protected Geographical Indication) GGA Global Gecko Association GGA Georgia Geocachers Association GC-3') and yielded a 260-bp product. Forty cycles of amplification were carried out for both rounds. The amplification products were analyzed by electrophoresis on a 1.5% agarose gel containing ethidium bromide, and the bands were visualized by UV light. To prevent false-positives from contamination, pipettes with filters were used in all manipulations. DNA extraction, preparation of the reaction mixture, PCR amplification, and detection were performed in different areas under a laminar flow hood. To detect any cross-contamination, all PCRs were performed with negative controls and sterile water. The products from nested PCR amplification were purified by using Sephacryl S-400 columns (Amersham Pharmacia Biotech AB, Uppsala, Sweden) and reamplified by using ABI Abi (ā`bī) [short for Abijah], in the Bible, King Hezekiah's mother. (Application Binary Interface) A specification for a specific hardware platform combined with the operating system. Prism dRhodamine Terminator Cycle Sequencing Ready Reaction Kit (PE Applied Biosystems, Foster City, CA, USA). Then, for each reaction, 5 [micro]L of PCR product, 4 [micro]L terminator-ready reaction mix, and 3 pmol of primer were added. The extension products were purified by ethanol precipitation to remove excess dye terminators. Each sample pellet was resuspended in 12.5 [micro] L of template suppression reagent and heated at 95[degrees]C for 3 min for denaturation denaturation, term used to describe the loss of native, higher-order structure of protein molecules in solution. Most globular proteins exhibit complicated three-dimensional folding described as secondary, tertiary, and quarternary structures. . Electrophoresis was carried out on the ABI prism 310 sequencer (PE Applied Biosystems) according to manufacturer's recommendations. The sequenced DNA fragments were analyzed by using Sequence Navigator v. 1.0.1 (PE Applied Biosystems). In the specimens of carriers, the R jirovecii dihydropteroate synthase (DHPS) locus was analyzed by PCR restriction fragment length polymorphism restriction fragment length polymorphism n. Abbr. RFLP Intraspecies variations in the length of DNA fragments generated by the action of restriction enzymes and caused by mutations that alter the sites at which these enzymes act, changing (RFLP RFLP abbr. restriction fragment length polymorphism RFLP restriction fragment length polymorphism. RFLP ), as previously described (28). In brief, the single-copy gene of DHPS was amplified by the primers DHPS-3 (5'-GCG CCT CCT Circuit CCT Commission Canadienne du Tourisme (Canadian Tourism Commission) CCT Correlated Color Temperature CCT Common Customs Tariff (EU) CCT Certificate of Completion of Training ACA ACA - Application Control Architecture CAT ATT ATG ATG antithymocyte globulin. lymphocyte immune globulin (antithymocyte globulin equine, ATG, ATG equine, LIG) Atgam Pharmacologic class: Immunoglobulin Therapeutic class: Immunosuppressant GCC ATT TTA TTA Telecommunications Technology Association (Korea) TTA Teacher Training Agency (UK) TTA Triangle Transit Authority (Raleigh/Chapel Hill/Durham, North Carolina, USA) AAT C-3') and DHPS-4 (5'-GGA ACT TTC AAC (Advanced Audio Coding) An audio compression technology that is part of the MPEG-2 and MPEG-4 standards. AAC, especially MPEG-4 AAC, provides greater compression and better sound quality than MP3, which also came out of the MPEG standard. TTG tTG Tissue Transglutaminase TTG Telltale Games (website) TTG TiVo To Go TTG Time-To-Go TTG Tonalite-Trondhjemite-Granodiorite TTG Tea Tree Gully (South Australia) TTG Tom Tom Go GCA ACC See adaptive cruise control. AC-3') by using a touchdown-PCR protocol, yielding a 370-bp fragment. The PeR product was divided into 3 aliquots. One was used to confirm the presence of a 370-bp fragment from the DHPS gene. The second and third aliquots were used to identify wild-type sequences versus mutations in codons 55 and 57 by RFLP with Accl and HaeIII (Roche Diagnostics, Mannheim, Germany), respectively. When the mutation is present, a 370-bp band appears. After RFLP in wild-type samples, bands appear at 229 bp and 141 bp with AccI and at 221 bp and 149 bp with HaeIII. Laboratory Studies Peripheral blood lymphocyte subsets were determined by using a flow cytometer (Cytoron Absolute, Ortho, Raritan, N J, USA) after incubation with monoclonal antibodies OKT OKT Oktober (German: October) OKT Amiga Oktalyzer (digital music file format) OKT Orang Kena Tuduh (Malaysia court cases) 3, OKT4, and OKT8 (Ortho). Serum anti-HIV antibodies were determined by a commercial enzyme-linked immunosorbent assay enzyme-linked immunosorbent assay n. ELISA. Enzyme-linked immunosorbent assay (ELISA) A diagnostic blood test used to screen patients for AIDS or other viruses. (ELISA ELISA (e-li´sah) Enzyme-Linked Immuno-Sorbent Assay; any enzyme immunoassay using an enzyme-labeled immunoreactant and an immunosorbent. ELISA n. ) (Multispot HIV HIV (Human Immunodeficiency Virus), either of two closely related retroviruses that invade T-helper lymphocytes and are responsible for AIDS. There are two types of HIV: HIV-1 and HIV-2. HIV-1 is responsible for the vast majority of AIDS in the United States. 1/HIV-2 rapid test, BioRad, Hercules, CA, USA). The results were interpreted according to the manufacturer's recommendations. Statistical Analysis The chi-square test was used for assessing differences between proportions. Results were considered significant at p < 0.05. Statistical analyses were performed by using the Statistical Package for Serial Studies for personal computers (SPSS A statistical package from SPSS, Inc., Chicago (www.spss.com) that runs on PCs, most mainframes and minis and is used extensively in marketing research. It provides over 50 statistical processes, including regression analysis, correlation and analysis of variance. version 12, SPSS Inc., Chicago, IL, USA). Results P. jirovecii DNA in 12 of 50 samples was successfully amplified twice by nested PeR. The mtLSU-rRNA fragment locus was successfully typed in 10 of the 12 samples in which mtLSU-rRNA had been amplified. Thus, R jirovecii carriage was detected in 20% of the participants. To assess the reproducibility and consistency of results, serial samples were obtained with a 2-day interval in 5 participants (1 carrier and 4 noncarriers). In all of them, consistent positive and negative patterns of results were obtained (positive PCR test after a positive result and negative PeR test after a negative result). The DHPS primer sets amplified a 370-bp band in 7 (70%) of 10 carriers. In all positive specimens with the DHPS-based PCR assay, the RFLP technique identified a wild DHPS genotype (Table). Results of physical examination were normal for Pneumocystis carriers. All were anti-HIV negative and had normal total lymphocyte and CD4+ cell counts. Chest radiographs were normal in 8 participants, and 1 participant had an apical cystic bullae bul·lae n. Plural of bulla. (Table). Only 1 person had taken steroids for a brief period in the 6 months before the study. No differences were detected due to age, sex, profession, alcohol intake, and smoking habit between R jirovecii carriers and noncarriers. Five known mtLSU-rRNA types are described for this Pneumocystis gene locus (15); 4 genotypes were isolated in the current study. Genotypes at this locus were identified on the basis of polymorphisms at nucleotide positions 85 and 248. Genotype 2 (85:A/248:C) was observed in 4 cases, genotype 1 (85:C/248:C) in 3 cases, genotype 3 (85:T/248:C) in 2 cases, and genotype 4 (85:C/248:T) in the remaining case (Table). During the follow-up, all carriers were asymptomatic for pulmonary disease. Pneumocystis DNA was detected by PCR in a second oropharyngeal wash obtained 6 months after the first in 2 (22.2%) of the 9 available carriers. Neither sample was typed because of insufficient quantity of PCR product. Discussion This study on immunocompetent healthy adults documents that P. jirovecii DNA can be detected by sensitive DNA amplification techniques by using noninvasive sampling of the respiratory tract. DNA detection does not establish the existence of infectious intact organisms. However, in animal models, detecting Pneumocystis DNA in nasal and oral samples is a good indicator that the organism is in the lung (29). Also, experiments show that Pneumocystis organisms can replicate in the lung alveolus alveolus (ălvē`ələs): see lungs. of immunocompetent hosts and remain infectious (30). Thus, our results agree with the hypothesis that the general human population could play an important role as a reservoir and source of R jirovecii infection and support the saprophytic saprophytic pertaining to saprophyte. nature of this pathogen in humans. An important finding of this study is that Pneumocystis DNA was not detected in >75% of the immunocompetent colonized adults within 6 months, which suggests the possible transience of the carrier state in healthy persons. This observation agrees with previous reports that show that most immunocompetent healthcare workers who were colonized with the pathogen cleared the infection (15,16). The number of persons examined in this study sufficiently demonstrated that P. jirovecii is an organism frequently found in healthy adults in the normal community. Since participants were all affiliated in some way with the Virgen del Rocio University Hospital in Seville, Spain, a broader group of healthy adults would need to be examined to estimate the prevalence of the carriers in the general population. Carrying out the study in a hospital could have somewhat biased the results, although we excluded persons with prior exposure to patients within the hospital and collected samples in a building outside the hospital. The accepted current diagnostic standard for Pneumocystis infection is the direct demonstration of the stained microorganism microorganism /mi·cro·or·gan·ism/ (-or´gah-nizm) a microscopic organism; those of medical interest include bacteria, fungi, and protozoa. in respiratory samples. Techniques based on PCR amplification of specific genome regions that provide high sensitivity are now widely used to diagnose several infectious diseases. These technical advances have allowed us to detect infections with samples obtained by noninvasive methods and in samples with low pathogen load. Different studies involving both sputum and bronchoalveolar lavage specimens have demonstrated the higher sensitivity of these techniques compared to conventional staining and monoclonal antibody immunohistochemical techniques (31,32). The main drawback to PCR is the possibility of false-positives (usually because of contamination) and the absence of rapid culture methods to confirm the PCR amplification results obtained. We avoided potential false-positives by adopting stringent precautionary measures and by examining the PCR signal from 2 different genes of P. jirovecii. The mtLSU-rRNA gene was selected for genotyping because it has a high degree of genetic conservation and is useful for detecting intraspecific in·tra·spe·cif·ic also in·tra·spe·cies adj. Arising or occurring within a species: intraspecific competition. differences between populations (33). The allelic frequency distribution patterns at this gene seen in the present study are similar to those reported in AIDS-associated PCP cases in a large study conducted in 5 cities in the United States (33). In that study, P. jirovecii genotypes were correlated with the place of diagnosis, rather than the person's place of birth. Our results support the concept of a community source of the infectious agents. Furthermore, an epidemiologic study was recently performed in patients in Spain with various pulmonary diseases. By also analyzing mtLSU-rRNA types, we found a high prevalence of genotype l (45%) and genotype 3 (40%) and lower of genotype 2 (10%) (28). In contrast, in the present study, genotype 2 was the most prevalent, whereas it was low in the pulmonary patient study, and genotype 3 was more frequently found in pulmonary patients than in normal healthy adults. Patients with pulmonary disorders may have a greater susceptibility to genotype 3. In our study, the rate of carriers identified as having the DHPS gene is 70%. The low amplification rate obtained is perhaps related to a low pathogen load in the samples. However, this rate is similar to that reported for AIDS patients with PCP in previously published studies (33). In the last decade, PCR technologies have shown that immunocompromised patients without PCP can be subclinically infected with Pneumocystis (19). In addition, a high prevalence of Pneumocystis is seen among immunocompetent patients with chronic pulmonary disorders (25,26,34), patients with small-cell lung carcinoma (35), or pregnant women (36). The pathogen has been detected in immunocompetent contacts of patients with PCP and in immunocompetent healthcare workers, whether or not they had contact with immunocompromised patients (15,16). Also, immunocompetent animal model hosts are commonly transiently colonized; Pneumocystis can replicate actively in their lungs and can be transmitted to another host (30,37). Moreover, postmortem lung screening using conventional staining for Pneumocystis showed small numbers of the organism in the lungs of immunocompetent individuals (38). Thus, substantial evidence exists of Pneumocystis colonization of healthy persons, and our findings are consistent with these observations. Most previous studies that failed to find the organism on autopsy (21) or in respiratory samples (14,29,31,36,39) from immunocompetent persons were performed on only a few persons. In some cases, failure was probably related to the use of either single PCR (31) or a less sensitive PCR (39). In others, failure could be related to the use of sputum or nasal secretions (14,29,36) that may have had lower numbers of organisms than in the oropharyngeal wash we analyzed or because of different procedures used for analyses (29). Protocols for acquiring and processing respiratory samples and analytical probes and methods should be standardized to enable better comparisons between studies performed in different laboratories. In summary, immunocompetent healthy adults might harbor short-lived infections that could be transmitted to other immunocompetent host in whom a transient infection can develop. Similarly, infants can become infected and a primary infection can develop, and immunosuppressed, susceptible people can become infected and clinical PCP can develop. Today, we know that human pneumocystosis is anthroponotic. Our findings may suggest that healthy adults represent a new dynamic reservoir and source of infection for human Pneumocystis species. Immunocompetent carriers in community ecosystems might present a public health issue that merits further research.
Table. Epidemiologic, biologic, and microbiologic
features of healthy Pneumocystis carriers *
Alcohol
Participant intake
(age [y], >40
sex) ([dagger]) Profession g/day
1 (28, F) Administrative No
2 (42, F) Administrative No
3 (43, F) Administrative No
4 (40, M) Administrative Yes
5 (41, F) New resident No
6 (27, F) New resident No
7 (32, F) New resident No
8 (40,M) University Yes
staff
9 (26, M) University Yes
staff
10 (42, M) University No
staff
Total
Participant lymphocyte
(age [y], Smoking count
sex) ([dagger]) habit (cells/[micro]L)
1 (28, F) No 2,327
2 (42, F) No 2,455
3 (43, F) No NA
4 (40, M) No 1,528
5 (41, F) No NA
6 (27, F) No 1,354
7 (32, F) No 2,300
8 (40,M) Yes 1,730
9 (26, M) Yes 3,602
10 (42, M) No 1,518
mtLSU-rRNA
genotype
Participant CD4+ cell (nucleotide
(age [y], count position:
sex) ([dagger]) (cells/[micro]L) identity)
1 (28, F) 653 3 (85:T/248:C)
2 (42, F) 1,168 1 (85:C/248:C)
3 (43, F) NA 4 (85:C/248:T)
4 (40, M) 520 3 (85:T/248:C)
5 (41, F) NA 2 (85:A/248:C)
6 (27, F) 550 2 (85:A/248:C)
7 (32, F) 604 1 (85:C/248:C)
8 (40,M) 924 2 (85:A/248:C)
9 (26, M) 924 2 (85:A/248:C)
10 (42, M) 432 1 (85:C/248:C)
DHPS genotype PCR result
Participant (codon position: at month
(age [y], identity) by PCR- 6 of
sex) ([dagger]) RFLP assay follow-up
1 (28, F) 1 (55:Thr/57:Pro) +
2 (42, F) 1 (55:Thr/57:Pro) -
3 (43, F) Not amplified -
4 (40, M) Not amplified -
5 (41, F) 1 (55:Thr/57:Pro) NA
6 (27, F) 1 (55:Thr/57:Pro) -
7 (32, F) 1 (55:Thr/57:Pro) -
8 (40,M) 1 (55:Thr/57:Pro) +
9 (26, M) 1 (55:Thr/57:Pro) -
10 (42, M) Not amplified -
* mtLSU-rRNA, mitochondrial large subunit ribosomal RNA; DHPS,
dihydropteroate synthase; PCR, polymerase chain reaction, RFLP,
restriction fragment length polymorphism; F, female; M, male;
+, positive result, -, negative result; NA, not available.
([dagger]) Chest radiograph results were normal for all participants,
except participant 5, for whom results were not available, and
participant 9, who showed an apical cystic bullae.
Acknowledgment We thank Edna S. Kaneshiro for assistance during the preparation of the manuscript. This study was partially supported by the fifth Framework Program of the European Commission contract No. QLK2-2000-01369, the Research Project 32/02 of the Ministry of Health, Junta de Andalucia, and the Research Project FIS FIS n abbr (BRIT) (= Family Income Supplement) → ayuda estatal familiar 03/1743 of the Spanish Ministry of Health. Dr. Medrano is an instructor and fellow in the Department of Internal Medicine, Virgen del Rocio University Hospital, Seville, Spain. His main areas of interest include physiopathologic physiopathologic /phys·io·patho·log·ic/ (fiz?e-o-path?ah-loj´ik) pertaining to pathologic physiology. and epidemiologic research on human pathogens, such as Leishmania Leishmania /Leish·ma·nia/ (lesh-ma´ne-ah) a genus of parasitic protozoa, including several species pathogenic for humans. In some classifications, organisms are placed in four complexes comprising species and subspecies: L. and Pneumocvstis spp. References (1.) Stringer JR, Beard CB, Miller RF, Wakefield AE. A new name (Pneumocystis jirovecii) for Pneumocystis from humans. Emerg Infect Dis. 2002;8:891-6. (2.) Calderon-Sandubete EJ, Varela-Aguilar JM, Medrano-Ortega FJ, Nieto-Guerrero V, Respaldiza-Salas N, de la Horra-Padilla C, et al. Historical perspective on Pneumocystis carinii infection. Protist protist Any member of a kingdom (Protista) of diverse eukaryotes, including algae, protozoans, and lower fungi (see fungus). Most are single-celled organisms, though the algae tend to be multicellular. . 2002;153:303-10. (3.) Gigliotti F, Harmsen AG, Haidaris CG, Haidaris PJ. Pneumocystis carinii is not universally transmissible between mammalian species. Infect Immun. 1993;61:2886-90. (4.) Dei-Cas E. Pneumocystis infections: the iceberg? Med Mycol. 2000;38(Suppl 1):23-32. (5.) Meuwissen JHE Th, Tauber 1, Leeuwenberg ADEM ADEM Alabama Department of Environmental Management ADEM Administration de l'Emploi (Luxembourg) ADEM Acute Disseminated Encephalomyelitis ADEM Arkansas Department of Emergency Management ADEM Ateneo de Manila , Beckers PJA, Sieben M. Parasitologic and serologic observations of infection with Pneumocystis in humans. J Infect Dis. 1977:136:43-9. (6.) Pifer LL, Hughes WT, Stagno S, Woods D. Pneumocystis carinii infection: evidence for high prevalence in normal and immunosuppressed children. Pediatrics. 1978;61:354-1. (7.) Medrano FJ, Respaldiza N, Medrano A, Varela JM, Montes-Cano M, de La Horra C, et al. Seroprevalence seroprevalence Immunology The proportion of a population that is seropositive–ie, has been exposed to a particular pathogen or immunogen; the seropositivity of a population is calculated as the number of individuals who produce a particular antibody divided of Pneumocystis human infection in southern Spain. J Eukaryot Microbiol. 2003;50(Suppl): 649-50. (8.) Chen F, Gigliotti F, Harmsen AG. Latency is not an inevitable outcome of infection with Pneumocystis carinii. Infect Immun. 1993;6l:5406-9. (9.) O'Donnell WJ, Pieciak W, Chertow GM, Sanabria J, Lahive KC. Clearance of Pneumocystis carinii cystic in acute P. carinii pneumonia: assessment serial sputum induction. Chest. 1998;114:1264-8. (10.) Chaves JP, David S, Wauters JP, Van Melle G, Francioli P. Transmission of Pneumocystis carinii from AIDS patients to other immunosuppressed patients: a cluster of Pneumocystis carinii pneumonia Pneumocystis carinii pneumonia (PCP) A lung infection that affects people with weakened immune systems, such as people with AIDS or people taking medicines that weaken the immune system. Mentioned in: AIDS, Antiprotozoal Drugs, Sulfonamides in a renal transplant recipient. AIDS. 1991;5:927-32. (11). Vrathalitis I, Aoun M, Daneau D, Meunier F. Pneumocystis carinii pneumonia in patients with cancer. An increasing incidence. Cancer. 1993;71:481-5. (12.) Keely SP, Stringer JR, Baughman RP, Linke MJ, Walzer PD, Smulian AG. Genetic variation among Pneumocystis carinii hominis isolates in recurrent pneumocystosis. J Infect Dis. 1995;172:595-8. (13.) Keely SP, Stringer JR. Sequences of Pneumocystis carinii s.f hominis' strains associated with recurrent pneumonia vary at multiple loci. J Clin Microbiol. 1997;35:2745-7. (14.) Vargas SL, Ponce CA, Giglotti F, Ulloa AV, Prieto S, Munoz MP, et al. Transmission of Pneumocystis carinii DNA from a patient with P carinii pneumonia to immunocompetent contact health care workers. J Clin Microbiol. 2000;38:1536-8. (15.) Miller RF, Ambrose HE, Wakefield AE. Pneumocystis carinii f. sp hominis DNA in immunocompetent health care workers in contact with patients with P. carinii pneumonia. J Clin Microbiol. 2001 ;39:3877-82. (16.) Durand-Joly I, Soula F, Chabe M, Dalle JH, Lafitte JJ, Senechal M, et al. Long-term colonization with Pneumocystis jiroveeii in hospital staffs: a challenge to prevent nosocomial nosocomial /noso·co·mi·al/ (nos?o-ko´me-il) pertaining to or originating in a hospital. nos·o·co·mi·al adj. 1. Of or relating to a hospital. 2. pneumocystosis. J Eukaryot Microbiol. 2003;50(Suppl):614-5. (17.) Bartlett MS, Vermund SH, Jacobs R, Durant P J, Shaw MM, Smith JW, el al. Detection of Pneumocystis carinii DNA in air samples: likely environmental risk to susceptible persons. J Clin Microbiol. 1997;35:2511-3. (18.) Olsson M, Lidman C, Latouche S, Bjorkman A, Roux P, Linder E, et al. Identification of Pneumocystis carinii f. sp. hominis gene sequences in filtered air in hospital environments. J Clin Microbiol. 1998;36:1737-40. (19.) Nevez G, Raccurt C, Jounieaux V, Dei-Cas E, Mazars E. Pneumocystosis versus pulmonary Pneumocystis carinii colonization in HIV-negative and HIV-positive patients. AIDS. 1999;13:535-56. (20.) Peters SE, Wakefield AE, Sinclair K, Millard PR, Hopkin JM. A search for Pneumocystis carinii in postmortem lungs by DNA amplification. J Pathol. 1992;166:195-8. (21.) Wakefield AE, Pixley FJ, Banerji S, Sinclair K, Millard PR, Hopkin JM. Detection of Pneumocystis carinii with DNA amplification. Lancet. 1990;336:451-3. (22.) Vargas SL, Hughes WT, Santolaya ME, Ulloa AV, Ponce CA, Cabrera CE, et al. Search for primary infection by Pneumocystis carinii in a cohort of normal health children. Clin Infect Dis. 2001:32:855-61. (23.) Eisen D, Ross BC, Fairbairn J, Warren R J, Baird RW, Dwyer B. Comparison of Pneumocystis carinii detection by toluidine blue O to·lu·i·dine blue O n. A blue basic dye used as a heparin antagonist, an antibacterial agent, a nuclear and metachromatic stain, and a stain for electrophoretic analysis of RNA, RNase, and mucopolysaccharides. staining, direct immunofluorescence and DNA amplification in sputum specimens from HIV patients. Pathology. 1994:26:198-200. (24.) Helweg-Larsen J, Jensen JS, Benfield T, Svendsen UG, Lundgren JD, Lundgren B. Diagnostic use of PCR for detection of Pneumocystis carinii in oral wash samples. J Clin Microbiol. 1998;36:2068-72. (25.) Calderon EJ, Regordan C, Medrano FJ, Ollero M, Varela JM. Pneumocystis carinii infection in patients with chronic bronchial disease. Lancet. 1996;347:977. (26.) Sing A, Roggenkamp A, Autenricth IB, Heesemann J. Pneumocystis carinii carriage in immunocompetent patients with primary pulmonary disorders as detected by single or nested PCR. J Clin Microbiol. 1999;37:3409-10. (27.) Wakefield AE, Pixley FJ, Banerji S, Sinclair K, Miller RF, Moxon ER, et al. Amplification of mitochondrial ribosomal RNA sequences from Pneumocystis carinii DNA of rat and human origin. Mol Biochem Parasitol. 1990;43:69-76. (28.) Montes-Cano MA, de la Horra C, Martin-Juan J. Varela JM, Torronteras R, Respaldiza N, et al. Pneumocystis jiroveci genotypes in Spanish population. Clin Infect Dis. 2004;39:123-8. (29.) Oz HS, Hughes WT. DNA amplification of nasopharyngeal nasopharyngeal pertaining to the nasal and pharyngeal cavities. nasopharyngeal meatus see nasopharyngeal meatus. nasopharyngeal spasm see reverse sneeze. aspirates in rats: a procedure to detect Pneumocystis carinii. Microb Palhog. 1999;27:119-21. (30.) Chabe M, Dei-Cas E, Creusy C, Fleurisse L, Respaldiza N. Camus D, et al. Immunocompetent host as a reservoir of Pneumocystis organism: histological and RT-PCR RT-PCR reverse transcriptase-polymerase chain reaction. See PCR1. data demonstrate active replication. Eur J Clin Microbiol Infect Dis. 2004;23:89-97. (31.) Wakefield AE, Guiver L, Miller RF, Hopkin JM. DNA amplification on induced sputum samples for diagnosis of Pneumocystis carinii pneumonia. Lancet. 1991;337:1378-9. (32.) Leibovitz E, Pollack H, Moore T, Papellas J, Gallo L, Krasinski K, et al. Comparison of PCR and standard cytological staining for detection of Pneumocystis carinii from respiratory specimens from patients with or at high risk for infection by human immunodeficiency virus human immunodeficiency virus n. HIV. Human immunodeficiency virus (HIV) A transmissible retrovirus that causes AIDS in humans. . J Clin Microbiol. 1995;33:3004-7. (33.) Beard CB, Carter JL, Keely SP, Huang L, Pieniazek NJ, Moura INS, et al. Genetic variation in Pneumocystis carinii isolates from different geographic regions: implications for transmission. Emerg Infect Dis. 2000;6:265-72. (34.) Vargas SL, Ponce CA, Sanchez CA, Ulloa AV, Bustamante R, Juarez G. Pregnancy and asymptomatic carriage of Pneumocystis jiroveci. Emerg Infect Dis. 2003;9:605-6. (35.) Calderon EC, de la Horra C, Medrano FJ, Lopez-Suarez A, Montes-Cano M, Respaldiza N, et al. Pneumocystis jirovecii isolates with dihidropteroate synthase (DHPS) mutations in patients with chronic bronchial diseases. Eur J Clin Microbiol infect Dis. 2004;23:545-9. (36.) de la Horra C, Varela JM, Fernandez-Alonso J, Medrano FJ, Respaliza N, Montes-Cano M, et al. Association between human-Pneumocytis infection and small-cell lung carcinoma. Eur J Clin Invest. 2004;34:229-35. (37.) Dumolin A, Mazars E, Segury N, Gargallo-Viola V, Vargas S, Cailliez JC, et al. Transmission of Pneumocystis carinii disease from immunocompetent contacts of infected host to susceptible. Eur J Clin Microbiol Infect Dis. 2000;19:671-8. (38.) Sheldon WH. Subclinical subclinical /sub·clin·i·cal/ (sub-klin´i-k'l) without clinical manifestations. sub·clin·i·cal adj. Not manifesting characteristic clinical symptoms. Used of a disease or condition. Pneumocystis pneumonitis pneumonitis /pneu·mo·ni·tis/ (noo?mo-ni´tis) inflammation of the lung; see also pneumonia. hypersensitivity pneumonitis . Am J Dis Child. 1959;97:287-97. (39.) Atzori C, Agostine F, Angeli E, Mainini A, Orlando G, Cargnel A. Combined use of blood and oropharyngeal samples for noninvasive diagnosis of Pneumocystis pneumonia using the polymerase chain reaction. Eur J Clin Microbiol Infect Dis. 1998;17:241-6. Address for correspondence: Francisco J. Medrano, Department of Internal Medicine, Virgen del Rocio University Hospital, Avda Manuel Siurot s/n, 41013 Seville, Spain: tax: 34-95-501-4278; email: medrano@cica.es Francisco J. Medrano, * Marco Montes-Cano, * Manuel Conde, * Carmen de la Horra, * Nieves Respaldiza, * Antonia Gasch, * Maria J. Perez-Lozano, * Jose M. Varela, * and Enrique J. Calderon * * Virgen del Rocio University Hospital, Seville, Spain |
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