Lymph node biopsy specimens and diagnosis of cat-scratch disease.We report microbiologic analysis of 786 lymph node biopsy Lymph Node Biopsy Definition A lymph node biopsy is a procedure in which all or part of a lymph node is removed and examined to determine if there is cancer within the node. specimens from patients with suspected cat-scratch disease Cat-Scratch Disease Definition Cat-scratch disease is an uncommon infection that typically results from a cat's scratch or bite. Most sufferers experience only moderate discomfort and find that their symptoms clear up without any lasting harm after a (CSD CSD Commission on Sustainable Development CSD Serbian Dinar (ISO currency code) CSD Christopher Street Day CSD Circuit Switched Data (Sprint) CSD Computer Science Department CSD Community School District ). The specimens were examined by standard, cell culture, and molecular methods. Infectious agents were found in samples from 391 (49.7%) of 786 patients. The most commonly identified infectious agent was Bartonella henselae Bartonella henselae Rochalimaea henselae Infectious disease A slender, fastidious coccobacillary bacterium of the normal flora of cats associated with bacteremia, endocarditis, cat-scratch disease, bacillary angiomatosis, peliosis hepatis; it may affect (245 patients, 31.2%), the agent of CSD. Mycobacteriosis was diagnosed in 54 patients (6.9%) by culture and retrospectively confirmed by using a specific real-time PCR PCR polymerase chain reaction. PCR abbr. polymerase chain reaction Polymerase chain reaction (PCR) assay. 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. was diagnosed in 181 specimens suitable for histologic analysis (26.0%) from 47 patients. Moreover, 13 patients with confirmed Bartonella infections had concurrent mycobacteriosis (10 cases) or neoplasm (3 cases). A diagnosis of CSD does not eliminate a diagnosis of mycobacteriosis or neoplasm. Histologic analysis of lymph node biopsy specimens should be routinely performed because some patients might have a concurrent malignant disease or mycobacteriosis. ********** Lymph node lymph node Small, rounded mass of lymphoid tissue contained in connective tissue. They occur all along lymphatic vessels, with clusters in certain areas (e.g., neck, groin, armpits). enlargement is a common medical problem. Infections caused by bacterial, viral, and protozoal protozoal pertaining to or caused by protozoa. protozoal myeloencephalitis see equine protozoal myeloencephalitis. protozoal hepatitis caused usually by Toxoplasma, Neospora, Leishmania. agents are the most typical cause of localized lymphadenopathy lymphadenopathy /lym·phad·e·nop·a·thy/ (-op´ah-the) disease of the lymph nodes. angioimmunoblastic lymphadenopathy , angioimmunoblastic lymphadenopathy with dysproteinemia , but malignancies or lymphoproliferative diseases are also often found (1). Physicians must differentiate malignant lymphadenopathies or infectious diseases that require special care from benign reactive lymphadenopathy or self-limiting adenitis adenitis /ad·e·ni·tis/ (ad?e-ni´tis) inflammation of a gland. Bartholin adenitis inflammation of the greater vestibular gland (Bartholin's gland) resulting from acute infection of the gland. . In a large number of patients, the causes of lymphadenopathy remain undiagnosed. Causes of lymphadenopathy other than neoplasm that require urgent medical attention include tuberculosis and 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. infection. During the past 15 years, Bartonella henselae, the causative agent of cat-scratch disease (CSD), has been reported as a common cause of localized lymphadenopathy (1-3). Diagnostic techniques for Bartonella-related infections include culture of the pathogen (4,5), detection of organisms in lymph nodes Lymph nodes Small, bean-shaped masses of tissue scattered along the lymphatic system that act as filters and immune monitors, removing fluids, bacteria, or cancer cells that travel through the lymph system. by immunofluorescence Immunofluorescence A technique that uses a fluorochrome to indicate the occurrence of a specific antigen-antibody reaction. The fluorochrome labels either an antigen or an antibody. (6), molecular techniques including PCR amplification of Bartonella spp. genes (7,8), and 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. analysis (9,10). B. henselae is not commonly isolated from CSD patients (4,11), and PCR-based detection of various target genes of Bartonella species in tissue specimens has become the most widely accepted way of diagnosing CSD (7,8). Serologic analysis is a minimally invasive diagnostic technique that has been extensively evaluated for the diagnosis of CSD (9,10,12). The sensitivity of serologic tests varies from 1 laboratory to another, ranging from nearly 100% to <30% (9). Specificity may also vary, and a specificity [greater than or equal to] 95% may be achieved by using commercial tests with 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. cutoff titers [greater than or equal to] 128 (10). As a national reference center for rickettsioses Rickettsioses Often severe infectious diseases caused by several diverse and specialized bacteria, the rickettsiae and rickettsia-like organisms. The best-known rickettsial diseases infect humans and are usually transmitted by parasitic arthropod vectors. and bartonelloses, we routinely receive lymph node biopsy specimens from patients with suspected CSD. In this study, we analyzed a large collection of lymph node biopsy samples obtained from January 2001 through August 2005 using microbial microbial pertaining to or emanating from a microbe. microbial digestion the breakdown of organic material, especially feedstuffs, by microbial organisms. cultures (blood agar blood agar n. A nutrient culture medium that is enriched with whole blood and used for the growth of certain strains of bacteria. culture and cell culture) and 16S rDNA- and Bartonella-specific PCR. Our objective was to define the frequency of B. henselae and other bacterial infections in patients with suspected CSD in France. Methods Patients We studied lymph node biopsy specimens from patients with suspected CSD that were collected from January 2001 through August 2005. Tissues specimens sent to our reference center were obtained from both hospitalized patients and outpatients throughout France. We receive either the entire lymph node or a fragment of it; the specimens were sent either frozen or in transport media. This factor is crucial because most of the specimens received were not in suitable condition for histologic analysis. A definitive diagnosis of CSD was defined as a biopsy sample that was positive by PCR for 2 different target genes of Bartonella spp. (6). If a specimen had been previously analyzed and B. henselae was reported (7), the specimen was excluded from the present study. Detection of Bartonella 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 Tissue Specimens Total genomic DNA was extracted from samples with a QIAamp tissue kit (Qiagen, Hilden, Germany) as previously described (7). Samples were handled under sterile conditions to avoid cross-contamination. Genomic DNA was stored at 4[degrees]C until used as template in PCR assays. The primers used for B. henselae amplification and sequencing (internal transcribed spacer ITS (for internal transcribed spacer) refers to a piece of non-functional RNA situated between structural ribosomal RNAs (rRNA) on a common precursor transcript. Read from 5' to 3', this polycistronic rRNA precursor transcript contains the 5' external transcribed sequence (5' ETS), [ITS] region and pap31 gene) have been previously evaluated (6,7). Up to 10 samples were tested, along with negative controls (DNA from noninfected lymph nodes and sterile water) and a positive control (DNA from B. elizabethae for the ITS region, GenBank accession no. L35103, and DNA from B. henselae Houston-I for the pap31 gene, GenBank accession no. AF001274). Detection of Bacteria in Tissue Specimens Nucleic acids Nucleic acids The cellular molecules DNA and RNA that act as coded instructions for the production of proteins and are copied for transmission of inherited traits. were extracted with a QIAamp tissue kit (Qiagen) and PCR performed with universal 16S rDNA primers fD1 and rp2 (Eurogentec, Seraing, Belgium) (13) and Taq DNA polymerase DNA polymerase /DNA po·lym·er·ase/ (pah-lim´er-as) any of various enzymes catalyzing the template-directed incorporation of deoxyribonucleotides into a DNA chain, particularly one using a DNA template. (GIBCO-BRL Life Technologies, Gaithersburg, MD, USA). Amplification and sequencing of products were conducted as previously described (14). Up to 10 samples were tested, along with negative controls (noninfected lymph node and sterile water) and positive controls (B. henselae Houston-I and Staphylococcus aureus Staphylococcus au·re·us n. A bacterium that causes furunculosis, pyemia, osteomyelitis, suppuration of wounds, and food poisoning. Staphylococcus aureus Staphylococcus pyogenes (ATCC ATCC American Type Culture Collection, see there 29213). The 16S rDNA sequences obtained were compared with all bacterial 16S rRNA sequences available in the GenBank database by using the Blastn version 2.2.2 program (National Center for Biotechnology Information The National Center for Biotechnology Information (NCBI) is part of the United States National Library of Medicine (NLM), a branch of the National Institutes of Health. The NCBI is located in Bethesda, Maryland and was founded in 1988. , Bethesda, MD, USA). The efficiency of DNA extraction and presence of inhibitors in samples that were negative by PCR were tested by using primers that targeted a fragment of the human [beta]-globin gene as previously described (15). Detection of B. henselae in Lymph Nodes We confirmed B. henselae in lymph nodes of patients with CSD by using a specific monoclonal antibody monoclonal antibody, an antibody that is mass produced in the laboratory from a single clone and that recognizes only one antigen. Monoclonal antibodies are typically made by fusing a normally short-lived, antibody-producing B cell (see immunity) to a fast-growing for B. henselae as previously described (6). The slides were air-dried and fixed with methanol for 10 minutes at room temperature before testing with an immunofluorescence assay (6). The sensitivity and specificity of this assay and antibody were previously reported to be 79.6% and 92.5%, respectively (6). Culture Methods Lymph node biopsy specimens were placed on blood agar plates, incubated at 37[degrees]C in an atmosphere of 5% C[O.sub.2], and examined weekly for growth during a 2-month period. This process resulted in isolation of either Bartonella or mycobacteria mycobacteria members of the genus Mycobacterium. anonymous mycobacteria see opportunist (atypical) mycobacteria (below). nontubercular mycobacteria see opportunist (atypical) mycobacteria (below). (16). Specimens were also placed on human embryonic lung cells in shell vials and incubated at 37[degrees]C in an atmosphere of 5% C[O.sub.2] as previously described (4,17). From January 2002 to August 2005, specimens were also incubated onto horse blood agar supplemented with hemin hemin /he·min/ (he´min) 1. a porphyrin chelate of iron, derived from red blood cells; the chloride of heme. It is used to treat the symptoms of various porphyrias. 2. hematin (1). (100 mg/L). This procedure has been reported to improve the isolation rate of B. henselae and can also support growth of rapidly growing mycobacteria Mycobacteria that form colonies clearly visible to the naked eye in less than 7 days on subculture are termed rapid growers. List of rapidly growing Mycobacteria Nonchromogenic
1. lacking molecular oxygen. 2. growing, living, or occurring in the absence of molecular oxygen; pertaining to an anaerobe. conditions. Bartonella isolates were identified by PCR and sequencing as described above; other bacterial isolates were identified by using standard bacteriologic bac·te·ri·ol·o·gy n. The study of bacteria, especially in relation to medicine and agriculture. bac·te methods. Samples from which mycobacteria were isolated were reanalyzed retrospectively by real-time PCR with modified primers and probes targeting the ITS region as previously described (18). Histologic Analysis Samples that had not been frozen (181 specimens) were fixed in formalin formalin /for·ma·lin/ (for´mah-lin) formaldehyde solution. for·ma·lin n. An aqueous solution of formaldehyde that is 37 percent by weight. and processed for histologic analysis. Stains used included Gram, hematoxylin hematoxylin /he·ma·tox·y·lin/ (he?mah-tok´si-lin) an acid coloring matter from the heartwood of Haematoxylon campechianum; used as a histologic stain and also as an indicator. and eosin eosin /eo·sin/ (e´o-sin) any of a class of rose-colored stains or dyes, all being bromine derivatives of fluorescein; eosin Y, the sodium salt of tetrabromofluorescein, is much used in histologic and laboratory procedures. , periodic acid-Schiff per·i·od·ic acid-Schiff adj. Abbr. PAS Of, relating to, or being a reaction that tests for polysaccharides and related substances through the treatment of tissue sections with periodic acid stain and Schiff's reagent. , Ziehl-Neelsen, and Warthin-Starry. Statistical Analysis Two groups of patients were defined for demographic data comparisons: CSD patients (detection of Bartonella DNA) and non-CSD patients (no detection of Bartonella DNA). For data comparison, the Student t test or [chi square chi square (kī), n a nonparametric statistic used with discrete data in the form of frequency count (nominal data) or percentages or proportions that can be reduced to frequencies. ] test was performed by using EpiInfo version 6.0 software (Centers for Disease Control and Prevention Centers for Disease Control and Prevention (CDC), agency of the U.S. Public Health Service since 1973, with headquarters in Atlanta; it was established in 1946 as the Communicable Disease Center. , Atlanta, GA, USA). Results Diagnoses in Patients with Lymphadenopathy We tested 786 lymph node biopsy specimens from patients with suspected CSD. Only 181 specimens were suitable for histologic analysis. Neoplasm was diagnosed by histologic analysis in 47 (26.0%) of 181 patients (6 with skin carcinomas, 1 with acute leukemia acute leukemia Hematology A rapidly progressive malignancy of sudden onset, characterized by an uncontrolled 'clonal' proliferation of immature WBCs which replace BM and spill into the peripheral circulation; untreated AL may be fatal in wks to months. , 24 with lymphomas, 12 with Hodgkin disease, and 4 with Kaposi sarcoma Kaposi sarcoma Usually lethal cancer appearing as red-purple or blue-brown spots on the skin and other organs. It has been linked to one of the herpes viruses, and there is considerable debate about how it should be classified. ). Bacteria were cultured from 143 specimens (18.2%), and mycobacteria were the most frequently recovered organisms (54 [6.9%] of 786) on blood agar or by shell vial culture (Table 1). The 54 nodes that contained mycobacteria were retrospectively confirmed by using real-time PCR targeting the ITS region. Other common bacteria recovered either by culture or PCR were staphylococci (26 cases) and Propionibacterium Propionibacterium /Pro·pi·on·i·bac·te·ri·um/ (pro?pe-on?e-bak-ter´e-um) a genus of gram-positive bacteria found as saprophytes in humans, animals, and dairy products. Pro·pi·on·i·bac·te·ri·um n. aches (15 cases). B. henselae was cultured and successfully passaged from 1 lymph node, and B. quintana was cultured and amplified from 1 lymph node. Fastidious fas·tid·i·ous adj. 1. Possessing or displaying careful, meticulous attention to detail. 2. Difficult to please; exacting. 3. Having complex nutritional requirements. Used of microorganisms. bacteria were cultured from lymph nodes by the shell vial cell culture: 2 isolates of Coxiella burnetii Coxiella burnetii Infectious disease The single species of genus Coxiella, family Rickettsiaceae, a short, rod-shaped bacterium; it is global in distribution, causes Q fever, spreads by aerosol, primarily infects cattle, sheep, goats, multiplies well in the and 1 isolate of Francisella tularensis Francisella tu·la·ren·sis n. A bacterium of the genus Francisella that causes tularemia in humans. , which has been previously reported (19) (Table 1). Anaerobic bacteria Anaerobic bacteria Bacteria that do not require oxgyen, found in low concentrations in the normal vagina Mentioned in: Aminoglycosides, Bacterial Vaginosis, Flesh-Eating Disease, Periodontal Disease cultured from lymph nodes included Fusobacterium spp. (4 specimens), Prevotella sp. (1 specimen), and Clostridium perfringens Clostridium per·frin·gens or Clostridium welchii n. Gas bacillus. Clostridium perfringens Infectious disease An anaerobic gram-positive spore-forming rod, widely distributed in nature and present in the (1 specimen). Amplification of the 16S rDNA gene for common bacteria was performed on all specimens. Positive results were obtained for 236 patients (30.0%), and B. henselae was the most frequently amplified bacterium (122 cases, 51.7%). Other bacteria commonly detected included mycobacteria, staphylococci, streptococci Streptococcus (plural, streptococci) A genus of spherical-shaped anaerobic bacteria occurring in pairs or chains. Sydenham's chorea is considered a complication of a streptococcal throat infection. , and P. aches (Table 1). Fastidious bacteria were isolated from 5 lymph nodes: C. burnetii (3 cases), F. tularensis (1 case), and Tropheryma whipplei (1 case). These 5 diagnoses were confirmed by a second specific PCR with primers and probes routinely used in our laboratory. Using specific primers for the ITS region and pap31 gene of Bartonella spp., we identified Bartonella spp. in 245 patients (31.2%), including 122 patients identified by PCR with primers for the 16S rDNA gene. No discordance discordance /dis·cor·dance/ (dis-kord´ans) the occurrence of a given trait in only one member of a twin pair.discor´dant dis·cor·dance n. was observed between the ITS region and the pap31 gene. When compared with specific detection of Bartonella DNA, specificity of the 16S rDNA PCR was 100% but sensitivity was low (49.8%, 122 of 245 lymph nodes were positive). Positive and negative controls showed expected results in all tests. All but 1 of the sequences of the ITS region and pap31 genes we obtained were identical to those of B. henselae reported in GenBank. In 1 patient, the sequences obtained were identical to those of B. quintana. Among these 245 samples positive for Bartonella, 216 were also tested by direct immunofluorescence assay with monoclonal antibodies to B. henselae, of which 166 (76.9%) were positive. A total of 391 (49.7%) of 786 patients had an infectious disease Infectious disease A pathological condition spread among biological species. Infectious diseases, although varied in their effects, are always associated with viruses, bacteria, fungi, protozoa, multicellular parasites and aberrant proteins known as prions. (including the 10 patients whose specimens were B. henselae--positive by PCR and showed mycobacterial mycobacterial emanating from or pertaining to mycobacterium. mycobacterial granuloma may be caused by Mycobacterium tuberculosis (see cutaneous tuberculosis), M. infection), 47 had neoplasm (including 3 specimens with B. henselae--positive PCR result), and 351 (44.6%) had no identified cause for their lymphadenopathy (Table 1). On the basis of these results, we divided the patients into 2 groups: patients with a positive PCR result for Bartonella (n = 245) (CSD group) and the remaining patients (n = 541) (non-CSD group). Comparison of Demographic Data between Patient Groups The mean [+ or -] standard deviation In statistics, the average amount a number varies from the average number in a series of numbers. (statistics) standard deviation - (SD) A measure of the range of values in a set of numbers. (SD) age was 30.2 [+ or -] 20.4 years (range 1-94 years) in 245 patients with proven B. henselae or B. quintana lymphadenopathy (CSD group) versus 31.6 [+ or -] 20.7 years (range 4 months to 86 years) in the non-CSD group. Most patients with B. henselae CSD were <25 years of age (p = 0.032) (Figure 1). The mean [+ or -] SD ages of patients with neoplasm (46.2 [+ or -] 22.6 years, range 7-86 years) and mycobacterioses (39.5 [+ or -] 22.2 years, range 1-84 years) were greater than the mean [+ or -] SD age of patients with CSD (p<0.05 by Student t test) (Table 2). The sex ratio (male:female) was 1.28 in the CSD group and 1.50 in the non-CSD group, but this difference was not significant (p>0.05) (Table 2). In the CSD group, 89 of the lymph node biopsy specimens were from axillary nodes Axillary nodes Lymph nodes found in the armpit that drain the lymph channels from the breast. Mentioned in: Lymphedema (36.3%), 75 were from inguinal inguinal /in·gui·nal/ (in´gwi-n'l) pertaining to the groin. in·gui·nal adj. 1. Of or located in the groin. 2. nodes (30.6%), and 81 were from cervical nodes (33.1%). [FIGURE 1 OMITTED] We found that 13 of 245 patients with CSD had concurrent lymph node disease (Table 2). Ten had mycobacteriosis proven by culture (5 with M. tuberculosis, 3 with M. avium, 1 with M. fuerthenensis, and 1 with M. gordonae), and 3 had neoplasm (2 with lymphoma and 1 with Hodgkin disease). The mean [+ or -] SD age of these 13 patients (49.7 [+ or -] 16.0 years, range 27-72 years) was higher than the mean [+ or -] SD age of the remaining 232 patients with only CSD (p<0.05 by Student t test). Only 4 lymph node biopsy specimens from the 10 patients with concurrent mycobacteriosis were positive by Ziehl-Neelsen staining. Six of 10 lymph node biopsy specimens were positive in a direct immunofluorescence assay with monoclonal antibodies for B. henselae (Figure 2) as previously described (6). [FIGURE 2 OMITTED] Of the 3 patients with CSD and concurrent neoplasm, a positive PCR result for the 16S rDNA gene was obtained with DNA from 1 lymph node (B. henselae). Two of 3 lymph nodes were positive in a direct immunofluorescence assay with monoclonal antibodies to B. henselae as described previously (6). As expected, the number of patients with either mycobacteriosis or neoplasm in the non-CSD group was higher than in the CSD group (p = 0.014; n = 181 patients). Discussion Culture and PCR were used to examine lymph node biopsy specimens from patients with suspected CSD. These methods, i.e., blood agar and cell culture (20), molecular biology with PCR for the 16S rDNA gene (14), PCR with 2 specific genes from Bartonella (6, 7), and histologic analysis (20), have been previously validated and are routinely used for examination of lymph node samples: Our report describes an extensive study on lymph nodes using culture, 16S rDNA PCR amplification, and amplification of target genes of Bartonella spp. Our objective was to define all bacterial causes of lymphadenopathies for samples initially sent to our center for detection of CSD. In the patients we studied, 50% had infectious diseases, and the most common causative agent was B. henselae; [approximately equal to] 30% of suspected patients were PCR positive (CSD group). Sensitivity of PCR with the 16S 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 to diagnose CSD was lower than was Bartonella-specific PCRs. The sensitivity of PCR assays with the 16S rRNA gene for the diagnosis of CSD has been reported to vary from 43% to 100%, depending on the primers used and the definition of a positive case (21,22). In our laboratory, PCR with specific primers against Bartonella genes is more sensitive and specific in the diagnosis of CSD. In a recent study in Germany, B. henselae was the causative agent of head and neck lymphadenopathy in 61 (13.4%) of 454 patients (1). As in our study, B. henselae was the most common organism responsible for lymphadenopathy in adults and children (1). However, our higher percentage of positive PCR results was because specimens sent to our reference laboratory were from patients with suspected CSD. Many cases of CSD remain unrecognized because serologic or molecular analyses are not routinely used. We observed a low isolation rate for B. henselae on axenic axenic /axen·ic/ (a-zen´ik) not contaminated by or associated with any foreign organisms; used in reference to pure cultures of microorganisms or to germ-free animals. Cf. gnotobiotic. media or in cell culture, only 1 successfully passaged isolate among the 245 PCR-positive samples, which is consistent with previous findings (4,8). This rate did not improve when we used an enriched medium designed to improve isolation of B. henselae (11). A recently developed enriched liquid medium for growth of Bartonella strains (23) may be useful in obtaining more isolates of B. henselae from patients with CSD. However, in many lymph nodes negative by culture, we observed bacteria by direct immunofluorescence, which suggests that bacteria in lymph nodes are not viable (6). Consistent with this finding was that most nodes were necrotic at histopathologic examination (data not shown). One lymph node was positive for B. quintana by culture and PCR as previously reported (24). The long incubation time needed for isolation of Bartonella allows us to isolate mycobacterial strains by using blood agar culture (16). We found mycobacteria incidentally and not because of a specific search. Moreover, even if mycobacteria grew well in blood agar plates (16), sensitivity of culture from lymph nodes is not 100%. This fact means that the percentage of mycobacterial infections in our study was probably underestimated because specific PCR for mycobacteria was only performed retrospectively in culture-positive specimens. On the basis of these results, we now routinely perform Ziehl-Neelsen staining and PCR to detect mycobacteria in all specimens. Before the discovery of B. henselae and the use of PCR for its diagnosis, mycobacteria were the most frequent infectious agents causing lymphadenopathy (25), and staphylococci and group A streptococci were the main causes of acute adenitis. In our study, mycobacteria were the second most common infectious cause of lymph node enlargement; [greater than or equal to] 6.9% of patients were infected. The 16S rRNA PCR in our study had a lower sensitivity than culture in the diagnosis of mycobacterial infection. This finding may have resulted from sample pretreatment pretreatment, n the protocols required before beginning therapy, usually of a diagnostic nature; before treatment. pretreatment estimate, n See predetermination. to adequately purify DNA (26). Freidig et al. found that 24 (5.7%) of 419 lymph nodes were enlarged because of mycobacterial infection (Table 3) (27). Similar incidences have been reported by Doberneck (28) and Anthony and Knowles (29) (Table 3). Higher incidences of mycobacterial infections (27 [16.6%] of 163 lymph node biopsy specimens) were reported by Roberts and Linsey (25). In our study, 76% of mycobacterial infections were M. tuberculosis; 54% were M. tuberculosis in the study by Freidig et al. (27). This finding is consistent with the fact that the incidence of typical and atypical mycobacterial adenitis is age dependent; typical adenitis is more common in adults, and atypical adenitis is more common in children (30). Other agents found in our study were staphylococci and miscellaneous aerobic and anaerobic bacteria. Isolates of coagulase-negative staphylococci or P. acnes may be considered contaminants, but the remaining organisms are pathogens and should be considered causative agents of lymph node enlargement (31). We found that rare or fastidious organisms may be the cause of infectious adenitis. Such situations have been previously reported, especially infections with Nocardia spp. (32), C. burnetii (33), F. tularensis (34), or T. whipplei (35). Only because we used cell cultures in shell vials were we able to culture C. burnetii and F. tularensis in our study. Similarly, additional cases with these fastidious organisms, as well as 1 case of infection with T. whipplei, were diagnosed because of systematic use of broad-range PCR on lymph nodes. The cause of 351 cases of lymphadenopathy in this study could not be determined. Several reasons and limitations may explain this result. First, histologic data were obtained for only 23% of the lymph node specimens because most were sent to our center frozen or were too small. In 181 specimens, neoplasms may represent >25% of cases of suspected CSD. Thus, a similar proportion of neoplasms may be present in the remaining 605 specimens. For practical purposes, neoplasm can only be diagnosed by histopathologic analysis. Thus, lymph node excision is crucial in the diagnosis of malignant processes. Another limitation of our study was that we did not test for fungi or viruses that may also represent causes of lymphadenopathies. Mycobacterial infections in our study were diagnosed by culture and confirmed retrospectively by using a real-time quantitative PCR. We believe that the systematic use of real-time PCR for detection of mycobacteria will likely increase the percentage of such infections as causes of lymphadenopathies. Previous studies reported that the percentage of undiagnosed cases varied from 17.2% to 39.7% (Table 3), and malignant processes were more common than infectious diseases. In more recent studies, percentages of lymph node specimens with malignant processes were lower (11.5%-17.3%), and infectious diseases were more common (17.7%-48.6%) (1,8,36) (Table 3). We have showed that neoplasm could be clinically misdiagnosed as CSD. This finding was probably underestimated because we had previously analyzed lymph nodes only by culture and detection of fastidious organisms. Moreover, only flesh samples can be used in histologic analysis. Our results reemphasize that CSD may be misdiagnosed as neoplasm, and we believe that lymph node excision and histologic analysis are critical for accurate diagnosis. We found that 13 Bartonella-positive patients (4.2%) had concurrent disease; 10 had mycobacteriosis (Figure 2), and 3 had neoplasm. These patients were older than those with CSD alone. However, neoplasm and mycobacterial infection was less common in patients with CSD than in those without CSD (p = 0.014, n = 181 patients). In the only report of coincidental CSD and neoplasm, Ridder et al. found 2 patients with squamous cell carcinoma squamous cell carcinoma n. A carcinoma that arises from squamous epithelium and is the most common form of skin cancer. Also called cancroid, epidermoid carcinoma. and 2 patients with malignant B-cell lymphoma on the basis of high antibody titers to B. henselae (1). A high prevalence of B. henselae--specific antibodies in HIV-positive patients with generalized lymphadenopathy and patients with non-Hodgkin lymphoma has also been reported (37). Explanations for such associations are unknown, and the frequency of asymptomatic patients with CSD is not known. One may speculate that Bartonella infections produce more symptoms in patients with HIV infections, mycobacterial infections, or neoplasm or cause chronic infection in such cases. In conclusion, lymph node excision and testing by histologic analysis are critical in detecting malignant processes and mycobacterial infections, even in patients found to have CSD by PCR. A diagnosis of CSD does not preclude other concurrent diseases, and their presence should routinely be tested by histologic analysis. In addition to testing pus pus, thick white or yellowish fluid that forms in areas of infection such as wounds and abscesses. It is constituted of decomposed body tissue, bacteria (or other micro-organisms that cause the infection), and certain white blood cells. samples or serologic analysis, biopsy specimens should be examined by a histologist, as recently proposed for patients with lymphadenopathy (8,38,39). Our study also demonstrates the advantage of specific target gene amplification compared with 16S rDNA gene amplification. Moreover, physicians should be aware that CSD can occur concurrently with neoplasm and mycobacteriosis, especially in adults >49 years of age. Acknowledgments We thank Patrick Kelly and S. Hafenstein for reviewing the manuscript, P.E. Fournier and F. Fenollar for technical assistance, and all clinicians for helpful collaborations. References (1.) Ridder GJ, Boedeker CC, Technau-Ihling K, Grunow R, Sander A. Role of cat-scratch disease in lymphadenopathy in the head and neck. Clin Infect Dis. 2002;35:643-9. (2.) Carithers HA. Cat-scratch disease: an overview based on a study of 1,200 patients. Am J Dis Child. 1985;139:1124-33. (3.) Margileth AM. Antibiotic therapy for cat scratch disease cat scratch disease n. An infectious disease that may follow the scratch or bite of a cat, producing localized inflammation of lymph nodes and a low-grade fever. Also called benign inoculation lymphoreticulosis, cat scratch fever. : clinical study of therapeutic outcome in 268 patients and a review of the literature. Pediatr Infect Dis J. 1992;11:474-8. (4.) La Scola B, Raoult D. Culture of Bartonella quintana and Bartonella henselae from human samples: a 5-year experience (1993 to 1998). J Clin Microbiol. 1999;37:1899-905. (5.) Brenner SA, Rooney JA, Manzewitsch P, Regnery RL. Isolation of Bartonella (Rochalimaea) henselae: effects of methods of blood collection and handling. J Clin Microbiol. 1997;35:544-7. (6.) Rolain JM, Gouriet F, Enea M, Aboud M, Raoult D. Detection by immnnofluorescence assay of Bartonella henselae in lymph nodes from patients with cat scratch disease. Clin Diagn Lab Immunol. 2003;10:686-91. (7.) Zeaiter Z, Fournier PE, Raoult D. Genomic variation of Bartonella henselae strains detected in lymph nodes of patients with cat scratch disease. J Clin Microbiol. 2002;40:1023-30. (8.) Hansmann Y, DeMartino S, Piemont Y, Meyer N, Mariet P, Heller R, et al. Diagnosis of cat scratch disease with detection of Bartonella henselae by PCR: a study of patients with lymph node enlargement. J Clin Microbiol. 2005;43:3800-6. (9.) Sander A, Berner R, Ruess M. Serodiagnosis serodiagnosis /se·ro·di·ag·no·sis/ (-di?ag-no´sis) diagnosis of disease based on serologic tests.serodiagnos´tic se·ro·di·ag·no·sis n. pl. of cat scratch disease: response to Bartonella henselae in children and a review of diagnostic methods. Eur J Clin Microbiol Infect Dis. 2001;20:392-401. (10.) Maurin M, Rolain JM, Raoult D. Comparison of in-house and commercial slides for detection by immunofluorescence of immunoglobulins G and M against Bartonella henselae and Bartonella quintana. Clin Diagn Lab Immunol. 2002;9:1004-9. (11.) Fournier PE, Robson J, Zeaiter Z, McDougall R, Byrne S, Raoult D. Improved culture from lymph nodes of patients with cat scratch disease and genotypic characterization of Bartonella henselae isolates in Australia. J Clin Microbiol. 2002;40:3620-4. (12.) Regnery RL, Olson TG, Perkins BA, Bibb bibb n. 1. Nautical A bracket on the mast of a ship to support the trestletrees. 2. A bibcock. [Alteration of bib.] W. Serological serological pertaining to or emanating from serology. serological test one involving examination of blood serum usually for antibody. response to Rochalimaea henselae antigen in suspected cat-scratch disease. Lancet. 1992;339:1443-5. (13.) Weisburg WG, Barns SM, Pelletier DA, Lane DJ. 16S ribosomal DNA amplification for phylogenetic phy·lo·ge·net·ic adj. 1. Of or relating to phylogeny or phylogenetics. 2. Relating to or based on evolutionary development or history. study. J Bacteriol. 1991;173:697-703. (14.) Drancourt M, Bollet C, Carlioz A, Martelin R, Gayral JP, Raoult D. 16S ribosomal DNA sequence analysis of a large collection of environmental and clinical unidentifiable Adj. 1. unidentifiable - impossible to identify identifiable - capable of being identified bacterial isolates. J Clin Microbiol. 2000;38:3623-30. (15.) Fenollar F, Roux Roux , Pierre Paul Émile 1853-1933. French bacteriologist. His work with the diphtheria bacillus led to the development of antitoxins to neutralize pathogenic toxins. V, Stein A, Drancourt M, Raoult D. Analysis of 525 samples to determine the usefulness of PCR amplification and sequencing of the 16S rRNA gene for diagnosis of bone and joint infections. J Clin Microbiol. 2006;44:1018-28. (16.) Drancourt M, Carrieri P, Gevaudan M J, Raoult D. Blood agar and Mycobacterium tuberculosis: the end of a dogma. J Clin Microbiol. 2003;41:1710-1. (17.) Fournier PE, Drancourt M, Lepidi H, Gevaudan MJ, Raoult D. Isolation of mycobacteria from clinical samples using the centrifugation-shell vial technique. Eur J Clin Microbiol Infect Dis. 2000;19:69-70. (18.) Bruijnesteijn van Coppenraet ES, Lindeboom JA, Prins JM, Peeters MF, Claas EC, Kuijper EJ. Real-time PCR assay using fine-needle aspirates and tissue biopsy specimens for rapid diagnosis of mycobacterial lymphadenitis Lymphadenitis Definition Lymphadenitis is the inflammation of a lymph node. It is often a complication of a bacterial infection of a wound, although it can also be caused by viruses or other disease agents. in children. J Clin Microbiol. 2004;42:2644-50. (19.) Fournier PE, Bernabeu L, Schubert B, Mutillod M, Roux V, Raoult D. Isolation of Francisella tularensis by centrifugation Centrifugation A mechanical method of separating immiscible liquids or solids from liquids by the application of centrifugal force. This force can be very great, and separations which proceed slowly by gravity can be speeded up enormously in centrifugal of shell vial cell culture from an inoculation eschar eschar /es·char/ (es´kahr) 1. a slough produced by a thermal burn, by a corrosive application, or by gangrene. 2. tache noire. es·char n. . J Clin Microbiol. 1998;36:2782-3. (20.) Rolain JM, Chanet V, Laurichesse H, Beytout J, Raoult D. Cat scratch disease with vertebral ver·te·bral adj. 1. Of, relating to, or of the nature of a vertebra. 2. Having or consisting of vertebrae. 3. Having a spinal column. osteomyelitis osteomyelitis (ŏs'tēōmī'əlī`tĭs), infection of the bone and bone marrow. Direct infection of bone usually occurs through open fractures, penetrating wounds, or surgical operations. and spleen abscesses. Ann N Y Acad Sci. 2003;990:397-403. (21.) Sander A, Posselt M, Bohm N, Ruess M, Altwegg M. Detection of Bartonella henselae DNA by two different PCR assays and determination of the genotypes of strains involved in histologically defined cat scratch disease. J Clin Microbiol. 1999;37:993-7. (22.) Avidor B, Kletter Y, Abulafia S, Golan Y, Ephros M, Giladi M. Molecular diagnosis of cat scratch disease: a two-step approach. J Clin Microbiol. 1997;35:1924-30. (23.) Maggi RG, Duncan AW, Breitschwerdt EB. Novel chemically modified liquid medium that will support the growth of seven Bartonella species. J Clin Microbiol. 2005;43:2651-5. (24.) Raoult D, Drancourt M, Carta A, Gastaut JA. Bartonella (Rochalimaea) quintana isolation in patient with chronic adenopathy, lymphopenia, and a cat. Lancet. 1994;343:977. (25.) Roberts FJ, Linsey S. The value of microbial cultures in diagnostic lymph-node biopsy. J Infect Dis. 1984; 149:162-5. (26.) Noordhoek GT, Kolk AH, Bjune G, Catty cat·ty 1 adj. cat·ti·er, cat·ti·est 1. Subtly cruel or malicious; spiteful: a catty remark. 2. Catlike; stealthy. D, Dale JW, Fine PE, et al. Sensitivity and specificity of PCR for detection of Mycobacterium tuberculosis: a blind comparison study among seven laboratories. J Clin Microbiol. 1994;32:277-84. (27.) Freidig EE, McClure SP, Wilson WR, Banks PM, Washington JA. Clinical-histologic-microbiologic analysis of 419 lymph node biopsy specimens. Rev Infect Dis. 1986;8:322-8. (28.) Doberneck RC. The diagnostic yield of lymph node biopsy. Arch Surg. 1983;118:1203-5. (29.) Anthony PP, Knowles SA. Lymphadenopathy as a primary presenting sign: a clinicopathological study of 228 cases. Br J Surg. 1983;70:412-4. (30.) Lai KK, Stottmeier KD, Sherman IH, McCabe WR. Mycobacterial cervical lymphadenopathy. Relation of etiologic agents to age. JAMA JAMA abbr. Journal of the American Medical Association . 1984;251:1286-8. (31.) Ishige I, Usui Y, Takemura T, Eishi Y. Quantitative PCR of mycobacterial and propionibacterial DNA in lymph nodes of Japanese patients with sarcoidosis Sarcoidosis Definition Sarcoidosis is a disease which can affect many organs within the body. It causes the development of granulomas. Granulomas are masses resembling little tumors. They are made up of clumps of cells from the immune system. . Lancet. 1999;354:120-3. (32.) Newton JA Jr, Wallace MR. Nodular nodular marked with, or resembling, nodules. nodular dermatofibrosis see dermatofibrosis. nodular episcleritis see nodular fasciitis (below). nodular fasciitis a firm painless nodular swelling, 0. lymphadenitis caused by Nocardia brasiliensis. Clin Infect Dis. 1994;18:843. (33.) Tattevin P, Arvieux C, Dupont M, Guggenbuhl P, Lemeur A, Michelet C. (Whipple bacillus bacillus (bəsĭl`əs), any rod-shaped bacterium or, more particularly, a rod-shaped bacterium of the genus Bacillus. Some bacterium in the genus cause disease, for example B. ) in lymph nodes. Am J Med. 2002;113:334-6. (34.) Ellis J, Oyston PC, Green M, Titball RW. Tularemia tularemia (t  lərē`mēə) or rabbit fever, acute, infectious disease caused by Francisella tularensis (Pasteurella tularensis). . Clin
Microbiol Rev. 2002;15:631-46.(35.) Lepidi H, Costedoat N, Piette JC, Harle JR, Raoult D. Immunohistological detection of Tropheryma whipplei (Whipple bacillus) in lymph nodes. Am J Med. 2002; 113:334-6. (36.) Chau I, Kelleher MT, Cunningham D, Norman AR, Wotherspoon A, Trott P, et al. Rapid access multidisciplinary lymph node diagnostic clinic: analysis of 550 patients. Br J Cancer. 2003;88:354-61. (37.) Peter JB, Boyle M, Patnaik M, Hadfield TL, Barka NE, Schwartzman WA, et al. Persistent generalized lymphadenopathy Persistent generalized lymphadenopathy (PGL) A condition in which HIV continues to produce chronic painless swellings in the lymph nodes during the latency period. Mentioned in: AIDS persistent generalized lymphadenopathy 1. and non-Hodgkin's lymphoma in AIDS: association with Rochalimaea henselae infection. Clin Diagn Lab Immunol. 1994;1:115-6. (38.) Reynolds MG, Holman RC, Curns AT, O'Reilly M, McQuiston JH, Steiner CA. Epidemiology of cat-scratch disease hospitalizations among children in the United States. Pediatr Infect Dis J. 2005;24:700-4. (39.) Ben Ami R, Ephros M, Avidor B, Katchman E, Varon M, Leibowitz C, et al. Cat-scratch disease in elderly patients. Clin Infect Dis. 2005;41:969-74. Use of trade names is for identification only and does not imply endorsement by the Public Health Service or by the U.S. Department of Health and Human Services Noun 1. Department of Health and Human Services - the United States federal department that administers all federal programs dealing with health and welfare; created in 1979 Health and Human Services, HHS . Jean-Marc Rolain, * Hubert Lepidi, * Michel Zanaret, ([dagger]) Jean-Michel Triglia, ([double dagger]) Gerard Michel, ([section]) Pascal-Alexandre Thomas, ([paragraph]) Michele Texereau, # Andreas Stein, *** Anette Romaru, ([dagger]) ([dagger]) Francois Eb, ([double dagger])([double dagger]) and Didier Raoult * * Universite de la Mediterranee, Marseille, France; ([dagger]) Federation Oto-Rhingo-Laryngologie, Marseille, France; ([double dagger]) Hopital Timone Enfant, Marseille, France; ([section]) Hopital d'Enfants de la Timone, Marseille, France; ([paragraph]) Hopital Sainte-Marguerite, Marseille, France; #Federation de Medecine, Niort, France; ** Hopital de la Conception, Marseille, France; ([dagger]) ([dagger]) Laboratoire de Biologie, Niort, France; and ([double dagger]) ([double dagger]) Centre Hospitalier Universitaire, Amiens, France Dr Rolain is professor at the Unite des Rickettsies, the French national reference center for rickettsiosis rickettsiosis /rick·ett·si·o·sis/ (ri-ket?se-o´sis) infection with rickettsiae. rick·ett·si·o·sis n. Infection with Rickettsia bacteria. and the World Health Organization collaborative center in Marseille. His research interests include the study of emerging and reemerging bacteria and arthropodborne diseases. Address for correspondence: Didier Raoult, Unite des Rickettsies, Faculte de Medecine, 27 Bd Jean Moulin, 13385 Marseille CEDEX 5, France; email: Didier.Raoult@medecine.univ-mrs.fr
Table 1. Results of culture and PCR assays
of 786 biopsy lymph node specimens *
16S
Bartonella- rDNA-
Diagnosis or Positive positive positive
infection culture PCR PCR Total
CSD 1 244 122 244
Bartonella quintana 1 1 1 1
Q fever 2 0 3 3
Tularemia 1 0 1 1
Abiotrophia 2 0 2 2
adjacens
Actinomyces 1 0 1 1
Pasteurella 2 0 2 2
multocida
Mycobacterial 54 0 32 54
infection
Staphylococcus 16 0 16 16
aureus
Coagulase- 15 0 10 23
negative
Staphylococcus
Streptococcus 10 0 10 10
pyogenes
Fusobacterium spp. 4 0 4 4
Nocardia 1 0 1 1
asteroides
Propionibacterium 15 0 7 16
acnes
Prevotella sp. 1 0 1 1
Clostridium 1 0 1 1
perfringens
Tropheryma 0 0 1 1
whipplei
Miscellaneous 21 0 21 21
Neoplasm 0 0 0 47
Unknown 0 0 0 350
Total 148 245 236 449
* CSD, cat-scratch disease. Among 244 specimens PCR-positive
for B, henselae, 10 showed a concurrent mycobacterial
infection and 3 showed a neoplasm.
Table 2. Comparison of demographic data between
CSD patients and non-CSD patients *
Age, y
Factor No. patients (mean [+ or -] SD)
CSD group (total) 245 30.2 [+ or -] 20.4
CSD alone 231 29.4 [+ or -] 19.6
CSD plus mycobacteria 10 43.3 [+ or -] 8.2
CSD plus neoplasm 3 57.3 [+ or -] 6.0
Bartonella Quintana alone 1 31.6 [+ or -] 20.7
Non-CSD group 541 39.5 [+ or -] 22.2
Mycobacteria 44 46.2 [+ or -] 22.6
Neoplasm 44 30.2 [+ or -] 20.4
Sex ratio p value
Factor (M/F) ([dagger])
CSD group (total) 1.28
CSD alone 1.26
CSD plus mycobacteria 1.00
CSD plus neoplasm 3.00
Bartonella Quintana alone
Non-CSD group 1.50 >0.05
Mycobacteria 1.72 <0.05
Neoplasm 1.30 <0.05
* CSD, cat-scratch disease, SD, standard deviation.
([dagger]) Comparison of mean age of CSD group and
corresponding non-CSD group.
Table 3. Relevant studies of causes of lymphadenopathy, 1983-2006 *
Variable Doberneck (28) Roberts (25) Anthony (29)
Years 1972-1982 1978-1983 1983
No. patients 169 163 228
Mean age, y 34.6 (1-78) (1-90) (0-[greater
(range) than or
equal to] 60)
Infectious 8/79 (10.1) 76 11 (4.8)
diseases (%)
CSD (%) 0 0 3
Mycobacteria 5/79 (6.3) 27 (16.6) 6 (2.6)
(%)
Staphylococci or 3/79 41 NA
streptococci (%)
Malignant 119 (70.4) 51 (31.2%) 60 (26.3)
process (%)
Undiagnosed 42 (24.9) 28 (17.2) 68 (29.8)
(%)
Variable Freidig (27) Ridder (1)
Years 1978-1986 1997-2001
No. patients 419 454
Mean age, y 46.7 (2-89) 34.9 (2-90)
(range)
Infectious 66 (15.8) 156 (34.4)
diseases (%)
CSD (%) 0 61 (13.4)
Mycobacteria 24 (5.7) 5 (1.1)
(%)
Staphylococci or 2 13
streptococci (%)
Malignant 113 (27.0) 52 (11.5)
process (%)
Undiagnosed 113 (27.0) 171 (37.7)
(%)
Variable Chau (36) This study
Years 1996-2001 2001-2005
No. patients 423 786
Mean age, y 40 (14-90) 32.0 (1-94)
(range)
Infectious 75 (17.7) 391 (49.7)
diseases (%)
CSD (%) 3 245 (31.2)
Mycobacteria 12 (2.8) 54 (6.9)
(%)
Staphylococci or 2 49
streptococci (%)
Malignant 95 (17.3) 47 (26%)
process (%) ([dagger])
Undiagnosed 168 (39.7) 350 (44.6)
(%)
* CSD, cat-scratch disease.
([dagger]) Only 181 samples could be
tested by histopathologic analysis.
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