Clinical and epidemiological use of nested PCR targeting the repetitive element IS<i>1111</i> associated with the transposase gene from <i>Coxiella burnetii</i>

Mares-Guia, Maria Angélica M.M.; Guterres, Alexandro; Rozental, Tatiana; Ferreira, Michelle dos Santos; Lemos, Elba R.S.

doi:10.1016/j.bjm.2017.04.009

ABSTRACT

Q fever is a worldwide zoonosis caused by Coxiella burnetii—a small obligate intracellular Gram-negative bacterium found in a variety of animals. It is transmitted to humans by inhalation of contaminated aerosols from urine, feces, milk, amniotic fluid, placenta, abortion products, wool, and rarely by ingestion of raw milk from infected animals. Nested PCR can improve the sensitivity and specificity of testing while offering a suitable amplicon size for sequencing. Serial dilutions were performed tenfold to test the limit of detection, and the result was 10× detection of C. burnetti DNA with internal nested PCR primers relative to trans-PCR. Different biological samples were tested and identified only in nested PCR. This demonstrates the efficiency and effectiveness of the primers. Of the 19 samples, which amplify the partial sequence of C. burnetii, 12 were positive by conventional PCR and nested PCR. Seven samples—five spleen tissue samples from rodents and two tick samples—were only positive in nested PCR. With these new internal primers for trans-PCR, we demonstrate that our nested PCR assay for C. burnetii can achieve better results than conventional PCR.

Keywords:
Q fever; Coxiella burnetii; Molecular diagnosis; Nested PCR; IS1111

Introduction

Q fever is a worldwide zoonosis caused by Coxiella burnetii, a small obligate intracellular bacteria and Gram-negative pleomorphic member of the order Legionellales.¹1 Fournier PE, Marrie TJ, Raoult D. Minireview diagnosis of Q fever. J Clin Microbiol. 1998;36:1823-1834. It remains infectious in the environment for a long time and is resistant to chemical and physical factors.²2 Centers for Disease Control and Prevention. Q fever. Available from: http://www.cdc.gov/qfever/ http://www.cdc.gov/qfever/ http://www.cdc.gov/qfever/. Accessed 16.01.16.
http://www.cdc.gov/qfever/... The infection exists in a variety of animals including various ruminants, domestic and wild animals, birds, and arthropods (especially ticks).²2 Centers for Disease Control and Prevention. Q fever. Available from: http://www.cdc.gov/qfever/ http://www.cdc.gov/qfever/ http://www.cdc.gov/qfever/. Accessed 16.01.16.
http://www.cdc.gov/qfever/... Cattle, sheep, and goats are the primary reservoirs of C. burnetii.²2 Centers for Disease Control and Prevention. Q fever. Available from: http://www.cdc.gov/qfever/ http://www.cdc.gov/qfever/ http://www.cdc.gov/qfever/. Accessed 16.01.16.
http://www.cdc.gov/qfever/...

3 Angelakis E, Raoult D. Review Q fever. Vet Microbiol. 2010;140:297-309.

4 Fenollar F, Fournie PE, Raoult D. Molecular detection of Coxiella burnetii in the Sera of patients with Q fever endocarditis or vascular infection. J Clin Microbiol. 2004;42(11):4919-4924.^-⁵5 Maurin M, Raoult D. Q fever. Clin Microbiol Rev. 1999;12(4):518-553. Transmission to humans usually occurs through inhalation of contaminated aerosols from urine, feces, milk, amniotic fluid, placenta, abortion products, wool, or less commonly through ingestion of raw milk from infected animals.²2 Centers for Disease Control and Prevention. Q fever. Available from: http://www.cdc.gov/qfever/ http://www.cdc.gov/qfever/ http://www.cdc.gov/qfever/. Accessed 16.01.16.
http://www.cdc.gov/qfever/... ^,⁵5 Maurin M, Raoult D. Q fever. Clin Microbiol Rev. 1999;12(4):518-553.

There are various ways of detecting C. burnetii infection.³3 Angelakis E, Raoult D. Review Q fever. Vet Microbiol. 2010;140:297-309. Several PCR-based DNA detection methods have been used to diagnosis Q fever including conventional PCR, nested PCR, real-time PCR (qPCR), and the loop-mediated isothermal amplification (LAMP) assay.³3 Angelakis E, Raoult D. Review Q fever. Vet Microbiol. 2010;140:297-309.^,⁶6 Chen HW, Ching WM. Development of loop-mediated isothermal amplification assays for rapid and easy detection of Coxiella burnetii. J Microbiol Methods. 2014;107:176-181.^,⁷7 Klee SR, Tyczka J, Ellerbrok H, et al. Highly sensitive real-time PCR for specific detection and quantification of Coxiella burnetii. BMC Microbiol. 2006;6:2. Berri et al.⁸8 Berri M, Laroucau K, Rodolakis A. The detection of Coxiella burnetii from ovine genital swabs, milk and fecal samples by the use of a single touchdown polymerase chain reaction. Vet Microbiol. 2000;72:285-293. showed that the sensitivity of trans-PCR is 100-fold greater than that obtained by PCR using primer CB1-CB2. Complete sequencing of the C. burnetii genome showed 20 copies of the IS1111 transposase. There were many element number copies in the genome of C. burnetii, and this was a useful tool for the detection and differentiation of C. burnetii isolates.⁹9 Denison AM, Thompson HA, Massung RF. IS1111 insertion sequences of Coxiella burnetii: characterization and use for repetitive element PCR-based differentiation of Coxiella burnetii isolates. BMC Microbiol. 2007;7:91-98. The objective of this study was to increase the sensitivity of the trans-PCR primer using a nested PCR assay and to demonstrate its effectiveness in different species of animals and different types of samples.

Materials and methods

Clinical samples and DNA extraction

Patient samples (n = 24) with suspected Q fever were tested along with 68 domestic animals, 74 rodents, and 180 ticks from Rio de Janeiro, Brazil. Domestic animal samples and ticks were obtained from areas where C. burnetii infection was detected in human and animals,¹⁰10 Mares-Guia MAMM, Rozental T, Guterres A, et al. Molecular identification of the agent of Q fever - Coxiella burnetii - in domestic animals in State of Rio de Janeiro, Brazil. Rev Soc Bras Med Trop. 2014;47:231-234.

11 Lemos ER, Rozental T, Mares-Guia MA, et al. Q fever as a cause of fever of unknown origin and thrombocytosis: first molecular evidence of Coxiella burnetii in Brazil. Vector Borne Zoonotic Dis. 2011;11:85-87.^-¹²12 Mares-Guia MAMM, Rozental T, Guterres A, et al. Molecular Identification of Q Fever in Patients with a Suspected Diagnosis of Dengue in Brazil in 2013-2014. Am J Trop Med Hyg. 2016;94(5):1090-1094. and rodent samples were collected from various regions of Rio de Janeiro state as part of an ecological research project conducted on wild animals from 2008 and 2015. Conventional and nested PCR were used to assay biological specimens from the suspected Q fever cases as well as clot, tissue, milk, and anal and vaginal swab samples extracted from animals. In addition, tissue samples from rodents and ticks were also tested with conventional and nested PCR.

DNA was extracted from goats, sheep, rodents, dogs, and cats. Serum and clot samples were used for human DNA extraction. The samples were tested using a QIAamp DNA Mini Kit (Qiagen™, Valencia, CA, USA) according to the instruction manual. After extensive washing in PBS, the DNA from milk as well as anal and vaginal swabs was extracted using ATL (QIAamp DNA Mini Kit, Qiagen™) and proteinase K. Each sample (200 µL) was mixed directly with the ATL and proteinase K and incubated at 56 °C overnight. This was followed by an incubation step with AL buffer for 10 min at 70 °C.¹⁰10 Mares-Guia MAMM, Rozental T, Guterres A, et al. Molecular identification of the agent of Q fever - Coxiella burnetii - in domestic animals in State of Rio de Janeiro, Brazil. Rev Soc Bras Med Trop. 2014;47:231-234.^,¹³13 Rodolakis A, Berri M, Héchard C, et al. Comparison of Coxiella burnetii shedding in milk of dairy bovine, caprine, and ovine herds. J Dairy Sci. 2007;90:5352-5360. The extraction process continued with a QIAmp DNA kit (QIAamp DNA Mini Kit, Qiagen™) following the manufacturer's instructions. Negative controls were included in each extraction to check for possible DNA contamination.

Obtaining and purifying C. burnetii DNA

C. burnetii Nine Mile phase II strain isolate from the UNIFESP São Paulo Culture Collection was used as a the positive control.¹⁴14 Zamboni DS, Mortara RA, Rabinovitch M. Infection of Vero cells with Coxiella burnetii phase II: relative intracellular bacterial load and distribution estimated by confocal laser scanning microscopy and morphometry. J Microbiol Methods. 2001;43(3):223-232. According to Zamboni and collaborators, the stock suspensions containing the bacteria were mildly sonicated at 35 kHz for 15 min at room temperature to disrupt aggregates. C. burnetii were grown in Vero cells (about 3 × 10⁵ cells per 2 cm²). In 2-3 days, the Vero cells developed large vacuoles containing bacteria. There were 3-10 µL of bacterial stock per well. After 24 h, cultures were vigorously washed and fresh medium added (minimal essential medium, MEM, containing 15 mM 4-(2-hydroxy-ethyl)-1-piperazineethanesulfonic acid - HEPES, 2 g/L sodium bicarbonate, 1 mM L-glutamine and 5% (v/v) of fetal bovine serum).¹⁴14 Zamboni DS, Mortara RA, Rabinovitch M. Infection of Vero cells with Coxiella burnetii phase II: relative intracellular bacterial load and distribution estimated by confocal laser scanning microscopy and morphometry. J Microbiol Methods. 2001;43(3):223-232. The DNA was extracted from 200 µL of this solution using a QIAamp DNA Mini Kit (Qiagen™, Valencia, CA, USA) following the manufacturer's instructions. The DNA was then quantified and used as a positive control for the first PCR. Serial tenfold dilutions were used to examine the detection limit.

PCR assay

The PCR assay used a pair of primers that target the gene IS1111 transposase elements in the genome of C. burnetii.¹⁵15 Willems H, Thiele D, Frolich-Ritter R, Krauss H. Detection of Coxiella burnetii in cow's milk using the polymerase chain reaction (PCR). J Vet Med. 1994;41:580-587.^,¹⁶16 Hoover TA, Vodkin MH, Williams J. A Coxiella burnetii repeated DNA element resembling a bacterial insertion sequence. J Bacteriol. 1992;174:5540-5548. The expected amplification product using these primers was 687 bp. The pair of primers were Trans1 (5'TAT GTA TCC ACC GTA GCC AGT C-3') and Trans2 (5'-CCC AAC AAC ACC TCC TTATTC-3'). These primers were used to do a PCR reaction using 4 µL of each DNA sample in 25 µL final reaction volume. The final reaction mixture contained 1× PCR buffer 10×, 0.2 µM of each primer (RTD/Prodimol™, Belo Horizonte, MG, Brazil), 1.5 mM of MgCl₂, 200 µM of dNTP mix (20 mM of each deoxynucleotide triphosphate), 0.5 U of Platinum Taq DNA polymerase (Invitrogen™, Carlsbad, CA, USA), 4 µL of DNA sample, and nuclease-free water (Promega™, Madison, WI, USA). Amplification used a GeneAmp PCR System 9700 thermal cycler (Applied Biosystems™, Foster City, CA, USA): initial denaturation at 95 °C for 5 min, followed by 40 successive cycles of denaturation at 95 °C for 30 s, annealing at 60 °C for 30 s, and extension at 72 °C for 1 min. This was followed by a final extension of 7 min at 72 °C. All steps used negative controls to control contamination.

Nested PCR assay

Primers design

Oligonucleotide primers to detect C. burnetii were designed from conserved regions of different IS1111 gene sequences. The MUSCLE tool was used to perform multiple sequence alignment¹⁷17 Edgar RC. MUSCLE: a multiple sequence alignment method with reduced time and space complexity. BMC Bioinformatics. 2004;5:113.; MUSCLE is part of the MEGA 6 software package.¹⁸18 Tamura K, Stecher G, Peterson D, Filipski A, Kumar S. MEGA 6: molecular evolutionary genetics analysis version 6.0. Mol Biol Evol. 2013;30:2725-2729. The nucleotide sequences of the IS1111 gene were analyzed (GenBank accession no. AE016828, CP001020, CP001019, CP000890, CP000733, CP007555, HG825990, LK937696, and M80806). The highly conserved regions were identified, and the degenerate oligonucleotide primers were designed to correspond to nucleotides in these regions.

Standardization and gradient

We used primers from the trans-PCR for the first PCR; N3+ (5'-AAG CGT GTG GAG GAG CGA ACC-3') and N4- (5'-CTC GTA ATC ACC AAT CGC TTC GTC-3') were used for the second PCR designed from the gene IS1111 transposase elements in the genome of C. burnetii.¹⁵15 Willems H, Thiele D, Frolich-Ritter R, Krauss H. Detection of Coxiella burnetii in cow's milk using the polymerase chain reaction (PCR). J Vet Med. 1994;41:580-587.^,¹⁶16 Hoover TA, Vodkin MH, Williams J. A Coxiella burnetii repeated DNA element resembling a bacterial insertion sequence. J Bacteriol. 1992;174:5540-5548. The expected amplification product of the target sequence with these primers was 440 bp long. The 25 µL mixture contained 2 µL of DNA samples (2 µL of first PCR reaction mixture in second PCR). The final reaction mixture contained 1× PCR buffer 10×, 0.2 µM of each primer (RTD/Prodimol™, Belo Horizonte, MG, Brazil), 1.5 mM of MgCl₂, 200 µM of dNTP mix (20 mM of each deoxynucleotide triphosphate), and 0.5 U of Platinum Taq DNA polymerase (Invitrogen™, Carlsbad, CA, USA).

A gradient PCR amplification was performed in a Veriti 96-well thermal cycler (Applied Biosystems™, Foster City, CA, USA). This consisted of initial denaturation for 5 min at 95 °C, followed by 30 successive cycles of denaturation at 95 °C for 30 s, annealing in a gradient of 65/66/67/68/69/70 °C for 30 s, and extension at 72 °C for 1 min. This was followed by a final extension of 5 min at 72 °C. To confirm amplification, the products were analyzed by electrophoresis in 1% agarose gel stained with GelRed™ solution (Biotium, Hayward, CA, USA). A 100-bp DNA ladder (Invitrogen™, Carlsbad, CA, USA) served as a molecular weight marker. The amplified products were visualized under a UV light trans-illuminator and stored in a digital system for gel documentation (Carestream Gel Logic 212 Pro, Rochester, NY, USA) to select the annealing temperature. Thus, the selected reaction used initial denaturation for 5 min at 95 °C followed by 30 successive cycles of denaturation at 95 °C for 30 s, annealing at 66 °C for 30 s, extension at 72 °C for 30 s, and a final extension to 72 °C for 5 min.

Sensitivity of PCR and nested PCR assays

Vero cells with C. burnetii were extracted using the QIAamp DNA Mini Kit (Qiagen™, Valencia, CA, USA) following the manufacturer's instructions. After extraction, the total DNA was quantified using a Qubit^© 2.0 fluorometer (Invitrogen™, Carlsbad, CA, USA) indicating a concentration of 21.4 µg/mL. Solutions of purified C. burnetii were used as positive control, and dilutions were prepared ranging from 1 to 10.¹³13 Rodolakis A, Berri M, Héchard C, et al. Comparison of Coxiella burnetii shedding in milk of dairy bovine, caprine, and ovine herds. J Dairy Sci. 2007;90:5352-5360. Dilutions used 2 µL of the solution extracted with 18 µL of nuclease-free water until the 10¹³ dilution. Four µL of the DNA solution was used for the PCR, and 2 µL was used for the nested PCR assays.

Specificity of PCR and nested PCR assays

DNA samples of C. burnetii and 15 other bacteria were used in the PCR and the nested PCR assays to evaluate specificity. The bacteria were Rickettsia rickettsii, Rickettsia typhi, Ehrlichia chaffeensis, Ehrlichia canis, Anaplasma phagocytophilum, Bartonella henselae, Borrelia burgdorferi (Hantaviroses and Rickettsioses Laboratory, FIOCRUZ), Pseudomonas aeruginosa INCQS 00025 (ATCC 15442), Brucella abortus INCQS 00242 (ATCC 7705), Legionella pneumophila subsp. pneumophila INCQS 00451 (NCTC 11232 ATCC 33155), Staphylococcus aureus CCBH 3853 (ATCC 25923), Streptococcus pneumonia, Haemophilus influenzae, Neisseria meningitidis (Epidemiology and Molecular Systematics Laboratory, FIOCRUZ), and Listeria monocytogenes (Bacterial Zoonoses Laboratory, FIOCRUZ).

Results

Sensitivity of the PCR and nested PCR assays

Sensitivity was compared between the PCR and the nested PCR assays in the detection of C. burnetii DNA. The amplification product by PCR assay with the trans-PCR primers for the first PCR was detected until the 10⁸ dilution (Fig. 1). The first PCR data showed that the annealing temperature gradients were negative for solutions of 10⁹ to 10¹³. The detection by nested PCR assay with primers N3+ and N4- was effective to the 10⁹ dilution indicating that it is 10-fold more sensitive than the first PCR assay (Fig. 2). Thus, the selected reaction was the initial denaturation for 5 min at 95 °C followed by 30 successive cycles of denaturation at 95 °C for 30 s, annealing at 66 °C for 30 s, extension at 72 °C for 30 s, and a final extension to 72 °C for 5 min.

Fig. 1
PCR assay with C. burnetii performed with primers of first PCR as described in the materials and methods. Lanes: 1, negative control; 2, 100 bp DNA ladder; 3, C. burnetii suspension 1× [21.4 µg/mL]; 4, C. burnetii suspension 10×; 5, C. burnetii suspension 10²×; 6, C. burnetii suspension 10³×; 7, C. burnetii suspension 10⁴×; 8, C. burnetii suspension 10⁵×; 9, C. burnetii suspension 10⁶×; 10, C. burnetii suspension 10⁷×; 11, C. burnetii suspension 10⁸×; 12, C. burnetii suspension 10⁹×; 13, C. burnetii suspension 10¹⁰×; 14, C. burnetii suspension 10¹¹×; 15, C. burnetii suspension 10¹²×; and 16, C. burnetii suspension 10¹³×.

Fig. 2
PCR assay with C. burnetii performed with primers of nested PCR as described in the materials and methods. Lanes: 1, negative control of first PCR; 2, negative control of nested PCR; 3, 100 bp DNA ladder; 4, C. burnetii suspension 1×; 5, C. burnetii suspension 10×; 6, C. burnetii suspension 10²×; 7, C. burnetii suspension 10³×; 8, C. burnetii suspension 10⁴×; 9, C. burnetii suspension 10⁵×; 10, C. burnetii suspension 10⁶×; 11, C. burnetii suspension 10⁷×; 12, C. burnetii suspension 10⁸×; 13, C. burnetii suspension 10⁹×; 14, C. burnetii suspension 10¹⁰×; 15, C. burnetii suspension 10¹¹×; 16, C. burnetii suspension 10¹²×; and 17, C. burnetii suspension 10¹³×.

Specificity of PCR and nested PCR assays

DNA samples from the 15 other bacteria used in the first PCR and nested PCR assays to assess the specificity showed no amplification (data not shown).

Detection of C. burnetii DNA from clinical specimens

The samples were tested for C. burnetii DNA by the first PCR and the nested PCR assays. Of 24 patients, 2 were positive (clot sample). One sheep (tissue) and two dogs (blood samples) were also positive. Of 10 goats, six were positive (milk sample), and of 13 cats, one was positive (anal swab) (Table 1). Of 74 rodents, the spleen tissue sample from five rodents and two tick samples of the 180 tested (Table 2) were only positive with the nested PCR. Therefore, they were sequenced, and the partial sequences were deposited in GenBank.

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Table 1
Detection of Coxiella infection by PCR of primers (trans 1/2) and nested PCR (+N3/N4) among human, domestic animals, rodents, and tick samples collected in Rio de Janeiro between 2008 and 2015.

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Table 2
Partial sequences of the gene IS1111 transposase elements in the genome of C. burnetii at GenBank from samples obtained from nested PCR.

Other samples including milk, vaginal swab, tissue, and serum samples had initial PCRs that were positive. They were then sequenced using the nested PCR. The tissue sample from sheep (GenBank accession no. KC854154 - 373 bp), EDTA blood sample from dog (GenBank accession no. KT867377 - 439 bp), and fecal swab from cat (GenBank accession no. KC854155 - 394 bp) were also deposited in GenBank.

Discussion

PCR has been used widely for the diagnosis of infectious diseases including those caused by C. burnetti. Hemi-nested and nested PCR increase the sensitivity of PCR and lead to at least a 10,000-fold enhancement in PCR product over nonspecific products that could be co-amplified when using only the outer primers. The amount of PCR product used in the nested PCR should be adjusted according to the results of the first PCR. In future diagnostic work, all samples should be tested with nested primers regardless of the first PCR result. False negative results after the first PCR could occur due to a very small number of copies.¹⁹19 Klein D. Quantification using real-time PCR technology: applications and limitations. Trends Mol Med. 2002;8(6):257-260.^,²⁰20 Watzinger F, Ebner K, Lion T. Detection and monitoring of virus infections by real-time PCR. Mol Aspects Med. 2006;27(2-3):254-298.

The objective of this study was to design and use nested PCR for a target gene that has already been shown to have sufficient specificity and sensitivity.⁸8 Berri M, Laroucau K, Rodolakis A. The detection of Coxiella burnetii from ovine genital swabs, milk and fecal samples by the use of a single touchdown polymerase chain reaction. Vet Microbiol. 2000;72:285-293.^,¹⁵15 Willems H, Thiele D, Frolich-Ritter R, Krauss H. Detection of Coxiella burnetii in cow's milk using the polymerase chain reaction (PCR). J Vet Med. 1994;41:580-587.^,¹⁶16 Hoover TA, Vodkin MH, Williams J. A Coxiella burnetii repeated DNA element resembling a bacterial insertion sequence. J Bacteriol. 1992;174:5540-5548. These new internal primers for trans-PCR proved that there was a 10× increase in sensitivity with an optimal sequence size of 440 bp.

Although Boden and colleagues developed Nested PCR using the IS1111 element as the target,²¹21 Boden K, Wagner-Wiening C, Seidelc T, et al. Diagnosis of acute Q fever with emphasis on enzyme-linked immunosorbent assay and nested polymerase chain reaction regarding the time of serum collection. Diagn Microbiol Infect Dis. 2010;68:110-116. our study verified not only the presence of the partial sequence of the C. burnetii gene in serum samples but also used it to test for other samples used for epidemiological studies such as swabs, milk, and ticks. Samples for epidemiological research may have small amounts of microorganisms.²²22 de Bruin A, de Groot A, de Heer L, et al. Detection of Coxiella burnetii in complex matrices by using multiplex quantitative PCR during a major Q fever outbreak in The Netherlands. Appl Environ Microbiol. 2011;77:6516-6523. In contrast to Duron,²³23 Duron O. The IS1111 insertion sequence used for detection of Coxiella burnetii is widespread in Coxiella-like endosymbionts of ticks. FEMS Microbiol Lett. 2015;362:fnv132. http://dx.doi.org/10.1093/femsle/fnv132.
http://dx.doi.org/10.1093/femsle/fnv132... small size amplifications can actually characterize the detection of fragments and not C. burnetii in its whole form. Thus, we developed this primer, which is located at a different site and with a reasonable size for sequencing. We determined that our amplicons were different from the qPCR DNA sequences studied previously.²⁴24 Pearson T, Cocking JH, Hornstra HM, Keim P. False detection of Coxiella burnetii—what is the risk? FEMS Microbiol Lett. 2016;363:fnw088. http://dx.doi.org/10.1093/femsle/fnw088.
http://dx.doi.org/10.1093/femsle/fnw088... The primers developed in the present study are not likely to result in amplification of endosymbionts due to the degradation in this particular region of their IS1111 gene.²⁴24 Pearson T, Cocking JH, Hornstra HM, Keim P. False detection of Coxiella burnetii—what is the risk? FEMS Microbiol Lett. 2016;363:fnw088. http://dx.doi.org/10.1093/femsle/fnw088.
http://dx.doi.org/10.1093/femsle/fnw088...

Pearson and colleagues²⁴24 Pearson T, Cocking JH, Hornstra HM, Keim P. False detection of Coxiella burnetii—what is the risk? FEMS Microbiol Lett. 2016;363:fnw088. http://dx.doi.org/10.1093/femsle/fnw088.
http://dx.doi.org/10.1093/femsle/fnw088... detected Coxiella-like bacteria through the IS1111 target. These are rare in tick populations, which limits the impact of false positives on prevalence estimates of C. burnetii. We distinguished C. burnetii from Coxiella-like bacteria using C. burnetii SNP genotyping assays due to the extreme sensitivity of the IS1111 multiple copy assay.

Although several qPCR techniques have been shown to be sensitive for diagnosis,³3 Angelakis E, Raoult D. Review Q fever. Vet Microbiol. 2010;140:297-309.^,⁷7 Klee SR, Tyczka J, Ellerbrok H, et al. Highly sensitive real-time PCR for specific detection and quantification of Coxiella burnetii. BMC Microbiol. 2006;6:2. this study aimed to find an alternative to conventional PCR in laboratories with few applicable financial resources for the realization of a qPCR. Chen et al. also proposed a novel detection method for serum samples.⁶6 Chen HW, Ching WM. Development of loop-mediated isothermal amplification assays for rapid and easy detection of Coxiella burnetii. J Microbiol Methods. 2014;107:176-181. However, nested PCR can be used in different types of samples such as milk, swabs, and tissue samples.²⁵25 Kim SG, Kim EH, Lafferty CJ, et al. Coxiella burnetii in bulk tank milk samples, United States. Emerg Infect Dis. 2005;11:619-621.

Recently, the presence of IS1111 in both C. burnetii and in the Coxiella-like endosymbionts led to questioning the specificity of the diagnostic tests in Q fever epidemiology. However, IS1111 amino-acid sequences in Coxiella-like endosymbionts revealed the presence of degraded sequences containing an internal stop codon(s). These are likely non-functional.²³23 Duron O. The IS1111 insertion sequence used for detection of Coxiella burnetii is widespread in Coxiella-like endosymbionts of ticks. FEMS Microbiol Lett. 2015;362:fnv132. http://dx.doi.org/10.1093/femsle/fnv132.
http://dx.doi.org/10.1093/femsle/fnv132... Thus, PCR or qPCR techniques for Q fever diagnosis using small fragments of the IS1111-DNA may lead to misidentification.²¹21 Boden K, Wagner-Wiening C, Seidelc T, et al. Diagnosis of acute Q fever with emphasis on enzyme-linked immunosorbent assay and nested polymerase chain reaction regarding the time of serum collection. Diagn Microbiol Infect Dis. 2010;68:110-116. Conversely, our new internal primers (N4-) for IS were developed considering the degraded regions for Coxiella-like endosymbionts. Therefore, we provide a nested PCR technique with better sensitivity for C. burnetii and a suitable DNA fragment size for genetic characterization.

Using these primers, we amplified and sequenced 440 bp partial sequences that do not align with the 15 other bacteria tested here. This makes the primers a great alternative for qPCR. We also used samples from different hosts and different types, and we improved the specificity of the amplified material. In animals, we identified positive cases in sample types other than blood. This makes this technique valuable for surveillance. We demonstrated that our nested PCR assay for C. burnetii achieved better results than conventional PCR and that this method may be a good alternative for the diagnosis of C. burnetii infection.

Financial support

This study was supported by FIOCRUZ and grants from Conselho Nacional para o Desenvolvimento Cientifico e Tecnológico (CNPq) Project 407664/2012 and Fundação de Amparo à Pesquisa do Estado do Rio de Janeiro (FAPERJ), Project E-26/010.001567/2014.

Acknowledgments

Phase II Nine Mile strain of C. burnetii was provided by Dr. Fernando Real and Dr. Alexis Melo from EPM, UNIFESP, São Paulo, SP, Brazil. Bacterial DNA was kindly provided by Dr. Ivano de Filippis, Collection Reference Microorganisms in Health Surveillance, CMRVS Fundação Oswaldo Cruz - FIOCRUZ, Brazil; the Epidemiology and Molecular Systematics Laboratory - Fundação Oswaldo Cruz - FIOCRUZ, Brazil; and Dra. Martha Pereira, Bacterial Zoonoses Laboratory - Fundação Oswaldo Cruz - FIOCRUZ, Brazil.

References

¹
Fournier PE, Marrie TJ, Raoult D. Minireview diagnosis of Q fever. J Clin Microbiol 1998;36:1823-1834.
²
Centers for Disease Control and Prevention. Q fever. Available from: http://www.cdc.gov/qfever/ http://www.cdc.gov/qfever/ http://www.cdc.gov/qfever/ Accessed 16.01.16.
» http://www.cdc.gov/qfever/
³
Angelakis E, Raoult D. Review Q fever. Vet Microbiol 2010;140:297-309.
⁴
Fenollar F, Fournie PE, Raoult D. Molecular detection of Coxiella burnetii in the Sera of patients with Q fever endocarditis or vascular infection. J Clin Microbiol 2004;42(11):4919-4924.
⁵
Maurin M, Raoult D. Q fever. Clin Microbiol Rev 1999;12(4):518-553.
⁶
Chen HW, Ching WM. Development of loop-mediated isothermal amplification assays for rapid and easy detection of Coxiella burnetii J Microbiol Methods 2014;107:176-181.
⁷
Klee SR, Tyczka J, Ellerbrok H, et al. Highly sensitive real-time PCR for specific detection and quantification of Coxiella burnetii BMC Microbiol 2006;6:2.
⁸
Berri M, Laroucau K, Rodolakis A. The detection of Coxiella burnetii from ovine genital swabs, milk and fecal samples by the use of a single touchdown polymerase chain reaction. Vet Microbiol 2000;72:285-293.
⁹
Denison AM, Thompson HA, Massung RF. IS1111 insertion sequences of Coxiella burnetii: characterization and use for repetitive element PCR-based differentiation of Coxiella burnetii isolates. BMC Microbiol 2007;7:91-98.
¹⁰
Mares-Guia MAMM, Rozental T, Guterres A, et al. Molecular identification of the agent of Q fever - Coxiella burnetii - in domestic animals in State of Rio de Janeiro, Brazil. Rev Soc Bras Med Trop 2014;47:231-234.
¹¹
Lemos ER, Rozental T, Mares-Guia MA, et al. Q fever as a cause of fever of unknown origin and thrombocytosis: first molecular evidence of Coxiella burnetii in Brazil. Vector Borne Zoonotic Dis 2011;11:85-87.
¹²
Mares-Guia MAMM, Rozental T, Guterres A, et al. Molecular Identification of Q Fever in Patients with a Suspected Diagnosis of Dengue in Brazil in 2013-2014. Am J Trop Med Hyg 2016;94(5):1090-1094.
¹³
Rodolakis A, Berri M, Héchard C, et al. Comparison of Coxiella burnetii shedding in milk of dairy bovine, caprine, and ovine herds. J Dairy Sci 2007;90:5352-5360.
¹⁴
Zamboni DS, Mortara RA, Rabinovitch M. Infection of Vero cells with Coxiella burnetii phase II: relative intracellular bacterial load and distribution estimated by confocal laser scanning microscopy and morphometry. J Microbiol Methods 2001;43(3):223-232.
¹⁵
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Edited by

Associate Editor: Roxane Piazza

Publication Dates

Publication in this collection
Jan-Mar 2018

History

Received
18 May 2016
Accepted
21 Apr 2017

This is an Open Access article distributed under the terms of the Creative Commons Attribution Non-Commercial No Derivative License, which permits unrestricted non-commercial use, distribution, and reproduction in any medium provided the original work is properly cited and the work is not changed in any way.

[1] Financial support

This study was supported by FIOCRUZ and grants from Conselho Nacional para o Desenvolvimento Cientifico e Tecnológico (CNPq) Project 407664/2012 and Fundação de Amparo à Pesquisa do Estado do Rio de Janeiro (FAPERJ), Project E-26/010.001567/2014.

Samples	PCR positive^a a Primers target the gene IS1111 transposase elements trans 1/trans 2. (No. tested)	Nested PCR positive^b b Primers target the gene IS1111 transposase elements of nested N3+/N4-. (No. tested)	Source location
Patients
Serum	0 (24)	0 (24)
Clot	2 (24)	2 (24)	Itaboraí, RJ

Sheep
Serum	0 (18)	0 (18)
Clot	0 (18)	0 (18)
Tissue	1 (1)	1 (1)	Itaboraí, RJ

Dogs
Serum	1 (19)	1 (19)
Clot	0 (19)	0 (19)
EDTA blood	1 (8)	1 (8)	Itaboraí, RJ
Vaginal swabs	0 (5)	0 (5)
Fecal swabs	0 (8)	0 (8)

Goats
Serum	0 (10)	0 (10)
Clot	0 (10)	0 (10)	Itaboraí, RJ
Milk	6 (7)	6 (7)
Vaginal swabs	0 (8)	0 (8)
Fecal swabs	0 (3)	0 (3)

Cats
Serum	0 (13)	0 (13)
Clot	0 (13)	0 (13)
Fecal swabs	1 (7)	1 (7)	Itaboraí, RJ

Rodents
Spleen tissue	0 (74)	5 (74)	Piraí/Valença, RJ

Ticks	0 (180)	2 (180)	Itaboraí, RJ

Register	Rodent/tick	Source material	Trans 1-2	N3+/N4-	GenBank accession number a(%); b(%)	Size (bp)
LBCE11866	Akodon cursor 1	Spleen	N	P	KT965026 a(100%); b(100%)	438
LBCE11914	Oligoryzomys nigripes	Spleen	N	P	KT965028 a(99%); b(100%)	326
LBCE11924	Mus musculus	Spleen	N	P	KT965029 a(100%); b(100%)	440
LBCE13257	Akodon cursor 2	Spleen	N	P	KT965030 a(100%); b(100%)	432
LBCE13265	Oxymycterus dasythricus	Spleen	N	P	KT965031 a(100%); b(100%)	440
C59	Rhipicephalus sanguineus	Tick	N	P	KT867378 a(100%); b(100%)	370
C154	Amblyomma sculptum	Tick	N	P	KT970067 a(99%); b(99%)	439

Brasil

Brasil

Clinical and epidemiological use of nested PCR targeting the repetitive element IS1111 associated with the transposase gene from Coxiella burnetii

ABSTRACT

Introduction

Materials and methods

Clinical samples and DNA extraction

Obtaining and purifying C. burnetii DNA

PCR assay

Nested PCR assay

Primers design

Standardization and gradient

Sensitivity of PCR and nested PCR assays

Specificity of PCR and nested PCR assays

Results

Sensitivity of the PCR and nested PCR assays

Specificity of PCR and nested PCR assays

Detection of C. burnetii DNA from clinical specimens

Discussion

Acknowledgments

References

Edited by

Publication Dates

History