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. 2020 Jan 3;2020:9814916. doi: 10.1155/2020/9814916

Real-Time PCR and Quantitative Culture for Mycoplasma pneumoniae Load in Pharyngeal Swabs from Children at Preliminary Diagnosis and Discharge

Fei Zhao 1, Xuemei Guan 2, Jing Li 3, Liyong Liu 1, Jie Gong 1, Lihua He 1, Fanliang Meng 1, Jianzhong Zhang 1,
PMCID: PMC6970502  PMID: 31998803

Abstract

Background

Extensive studies have focused on the diagnosis and treatment of Mycoplasma pneumoniae infection; however, rare studies investigated the posttreatment conditions. We analyzed the carrying status of M. pneumoniae in the respiratory tract of children before and after treatment.

Methods

Ninety-two children with M. pneumoniae pneumonia were included in this study. Clinical data were obtained from each patient, and pharyngeal swab sampling was performed at preliminary diagnosis and discharge. Real-time PCR and dilution quantitative culture were utilized to determine the DNA quantification and number of viable M. pneumoniae from samples collected upon preliminary diagnosis and discharge.

Results

All the 92 cases showed DNA positivity upon preliminary diagnosis, serum IgM antibody was detected in 80 patients, and positivity of M. pneumoniae culture was observed in 82 cases. Upon discharge, the M. pneumoniae nucleotide and culture positivity were detected in 87 and 49 cases, respectively. The content of viable M. pneumoniae was 10–104 CCU/mL and 10–102 CCU/mL in the preliminary diagnosis samples and discharge samples, respectively.

Conclusions

Real-time PCR was rapid and effective for the qualitative diagnosis of M. pneumoniae at the early stage, but it cannot be used to evaluate the prognosis of patients with M. pneumoniae infection. Quantitative analysis for M. pneumoniae DNA could not directly reflex the viable strain content.

1. Introduction

Mycoplasma pneumoniae is a major cause of respiratory tract infections in human, especially children and adolescents [1, 2]. It is responsible for about 10%–40% of the community acquired pneumonia (CAP) in children annually [3, 4]. In clinical practice, the agents used for treating M. pneumoniae infection mainly consist of macrolides, fluoroquinolones, and tetracycline antibiotics [5, 6]. Nowadays, macrolide antibiotics are preferred for treating M. pneumoniae infection in children with low toxicities, less adverse events, and high blood drug concentration [7, 8]. Although M. pneumoniae pneumonia (MPP) is usually considered a self-limited disease, it may trigger pulmonary complications that may progress into refractory M. pneumoniae pneumonia (RMPP), severe M. pneumoniae pneumonia (SMPP), and even lethal pneumonia [9, 10]. Meanwhile, some may present concurrent infection and multiple-organ infection, which results in poor prognosis [11, 12]. Therefore, M. pneumoniae infection is a heavy burden to the pediatric practice worldwide.

The diagnosis of M. pneumoniae infection in childhood is mainly relied on serology. In acute stage, the most frequently used method is based on determination of serum IgM antibody [13]. However, false-negativity may be generated in early stage in some patients due to poor IgM antibody titer. Then the second IgM antibody determination is necessary in a short term for the early diagnosis of cases suspected with RMPP [14]. Recently, nucleic acid amplification techniques (NAATs) represented by real-time PCR, with high sensitivity and specificity, have been gradually utilized in M. pneumoniae determination. Particularly, NAATs are crucial in early stage, in which the antibody titer is not adequate [15, 16].

The dissemination of viable M. pneumoniae is merely depending on aerosols, and infection models have been established in animals using aerosol inoculation [17]. Pathogens have been identified in the samples obtained from nose, throat, trachea, and sputum, which can be disseminated to a large scale through cough. Up to now, few studies have focused on the relationship between M. pneumoniae infection and dissemination. Meanwhile, rare studies have reported the prognosis of patients with M. pneumoniae infection after treatment [18]. Nilsson et al. [19] reported that M. pneumoniae DNA was still detected in the throat secretion in half of the patients about 7 weeks after disease onset. Moreover, certain cases showed persistent DNA positivity within several months. However, this scientific significance was hampered by the limitations of their study as the method could not tell the DNA of viable M. pneumoniae apart from nonviable ones [20]. Thus, methods that can accurately measure the amount of M. pneumoniae in throat are required to evaluate the clinical efficiency of treatment options. In this study, pharyngeal swab sampling was performed to the 92 children with M. pneumoniae pneumonia (MPP) before and after treatment, followed by real-time PCR, genotyping, and M. pneumoniae culture detection. We aim to investigate the carrier state of M. pneumoniae in the respiratory tract before and after treatment.

2. Material and Methods

2.1. Ethical Statement

Informed consent was obtained from at least one guardian of patients before enrolling this study. As the samples were collected in a noninvasive manner using a pharyngeal swab, the informed consent was obtained in an oral form from the guardian of each child. All the individuals were informed that the samples were only used for this clinical study. The study was approved by the Ethics Committee of the National Institute for Communicable Disease Control and Prevention, Chinese Center for Disease Control and Prevention (Beijing, China), and the Ethics Committee of the Affiliated Hospital of Beihua University (Jilin, China).

2.2. Patients

Ninety-two children with MPP admitted to Department of Pediatrics of Affiliated Hospital of Beihua University between January 2017 and March 2017 were included in this study. Patients with immune deficiency and/or received administration of antibiotics 2 weeks before diagnosis were excluded from this study. M. pneumoniae infection was diagnosed based on the demonstration of an IgM-specific anti-M. pneumoniae antibody titer of ≥1 : 160. All the patients received alternating treatment using intravenous injection of azithromycin (10 mg/kg, q.d., 5 days) and erythromycin (10 mg/kg, b.i.d., 3 days). All the patients were discharged from hospital upon remission of the symptoms, including elimination of positive signs and absorption of pulmonary lesions by chest film. After discharge, each patient was suggested to receive oral administration of azithromycin for 2-3 weeks.

2.3. Sample Collection

Pharyngeal swabs were collected from each patient upon preliminary diagnosis and labeled as A01 to A92, and upon discharge as B01 to B92, respectively. The samples were stored in Mycoplasma broth supplemented with 20% sterilized glycerol at −80°C upon collection and then transmitted to the National Institute for Communicable Disease Control and Prevention for subsequent analysis through cold chain ways.

2.4. Real-Time PCR

DNA was extracted from 200 μl samples using QIAamp DNA MINI kit (QIAGEN, No. 51306) according to the manufacturer's instructions. Quantitative real-time PCR was performed according to our previous description [21]. The amplification conditions were as follows: 95°C for 3 min, followed by 45 cycles of 95°C for 15 sec and 59°C for 30 sec. The standard curve was established using the standard concentration nucleotides (2 copies/μl to 2 × 106 copies/μl) of M. pneumoniae ATCC 29342 strain.

2.5. M. pneumoniae Culture and Identification of Clinical Samples

Clinical samples (200 μl) were inoculated on Mycoplasma selective broth medium (OXOID, Thermo Fisher, NY, USA) at 37°C. The ATCC 29342 strains served as the positive control, and the blank culture served as the negative control. The remaining samples were stored using an Eppendorf tube (200 μl) at −80°C until subsequent analysis. A yellow color on the medium with no turbidity was speculated to be M. pneumoniae positive. Bacterial contamination was considered in the presence of turbidity in the medium. The stored samples were subject to filtration using a 450 nm filter and then were cultured. Negativity was defined as no color changes within 5 weeks after culture. The color of medium was observed and the time interval between inoculation and M. pneumoniae positivity (TIIP) was recorded per day. Then 100 μl positive samples were inoculated on the selective agar medium. After culturing at 37°C for 1 week, the colonies were observed under a stereomicroscope. The typical colonies were passaged, followed by DNA extraction using QIAamp DNA MINI kit (Qiagen, No. 51306). Then passaged M. pneumoniae identification was conducted using real-time PCR as previously described [22].

2.6. M. pneumoniae Quantitative Culture of Clinical Samples

Quantitative culture analysis of M. pneumoniae was performed to the cultivate positive samples collected both upon preliminary diagnosis and discharge using the liquid broth medium dilution method by color-changing units (CCUs). The samples were subject to dilution culture (10×) in liquid medium (6 gradients for each sample; triplicate for each gradient) and cultured at 37°C. The ATCC 29342 strains served as the positive control, while the blank culture served as negative control. The number of viable M. pneumoniae was performed by determining the CCU value. Two pairs of samples presenting bacterial contamination (A26/B26 and A28/B28) were dropped out due to bias in the quantitative analysis generated in the presence of filtration of sample using a 450 nm filter.

2.7. Typing of Multiple-Locus Variable-Number Tandem-Repeat Analysis (MLVA)

M. pneumoniae positive samples upon preliminary diagnosis and discharge were selected for the MLVA typing. MLVA typing was performed according to the previous description with moderate modifications method [23, 24]. The DNA of each M. pneumoniae isolate was utilized as the template for Multiplex PCR amplification-linked capillary electrophoresis of four loci (i.e., Mpn13-16) selected for multilocus variable-number tandem-repeat (VNTR) analysis.

2.8. Statistical Analysis

All the data were entered into Excel 2007 sheet, and SPSS 17.0 software was utilized for the data analysis. Chi square test was performed for the nucleotide and culture positivity of M. pneumoniae upon preliminary diagnosis and discharge, as well as the bacterial contamination rate at these two time points. Paired Student's t-test was used for the comparison of DNA load and viable M. pneumoniae content upon preliminary diagnosis and discharge. P value of less than 0.05 was considered to be statistically significant.

3. Results

3.1. Clinical Characteristics of Patients

Ninety-two children (male: 65; female: 27; age: 5–15 years) were included in this study. The mean hospitalization duration was 10.7 days. The examination findings upon preliminary diagnosis were as follows: temperature, 38.33 ± 1.21°C; and white blood cell, 8.81 ± 2.40 cells/L. Among these patients, 83 (90.2%) showed cough, and 21 (22.8%) showed sputum. All the 92 cases (100%) showed shadows after X-ray. Serum M. pneumoniae IgM antibody was detected in 80 patients (87.0%), among which 12 were IgM-negative during the preliminary diagnosis. About 4–6 days after preliminary diagnosis, serum IgM antibody was performed to the 12 cases, and all of them were IgM-positive.

3.2. Real-Time PCR for the M. pneumoniae

No statistical differences were noticed in the detected DNA positivity of M. pneumoniae between that obtained upon preliminary diagnosis and that obtained upon discharge (100% vs. 94.6%, χ2 = 3.20, P > 0.05). M. pneumoniae DNA quantitative analysis indicated that the positive samples at the preliminary diagnosis showed no statistical differences compared with those obtained upon discharge (2.48 × 102–1.95 × 105 copies/mL vs. 1.86 × 102–6.70 × 105 copies/mL, t = 0.156, P > 0.05, Figure 1). The M. pneumoniae DNA quantity of 48 samples, including 5 negative samples, at preliminary diagnosis was higher than that at discharge. Twenty-eight samples showed comparable M. pneumoniae DNA quantity upon these two time points. The rest 16 samples showed lower M. pneumoniae DNA quantity at diagnosis compared to that of discharge. In each individual, elevation was defined as 2-fold increase in the DNA quantity.

Figure 1.

Figure 1

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Comparison of DNA load in the M. pneumoniae obtained from the pharyngeal swab in 92 cases upon preliminary diagnosis and discharge. ◆: M. pneumoniae negative culture samples. The numbers of samples were arranged in an ascending order based on the DNA load of preliminary diagnosis.

3.3. M. pneumoniae Culture

At preliminary diagnosis, the positivity for M. pneumoniae culture was significantly higher than that of discharge (89.1% vs. 53.2%, χ2 = 31.03, P < 0.05). For the preliminary diagnosis, the concordance rate of culture and nucleic acid detection was 89.1% among the 92 cases, while that at the discharge was 58.7%. Nine pharyngeal swabs (i.e., A14, A17, A20, A21, A26, A28, A41, A44, and A45) showed bacterial contamination during M. pneumoniae culture at the preliminary diagnosis. Only two swabs (i.e., B14 and B17) showed contamination at discharge. There were statistical differences between the contamination rates in the samples obtained upon two time points (χ2 = 5.14, P < 0.05). The DNA quantitative analysis and M. pneumoniae culture results of all samples were shown in Table 1.

Table 1.

Positive rates of samples with various M. pneumoniae DNA loads.

DNA load (copies/mL) Positivity
Preliminary diagnosis Discharge
<103 50.0% (1/2) 40.0% (6/15)
103–104 89.5% (51/57) 55.6% (25/45)
>104 91.0% (30/33) 66.7% (18/27)
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Five DNA negative samples were excluded. The positivity was defined as the ratio of positive samples to total samples.

3.4. MLVA Typing

In total, 49 pairs of samples were M. pneumoniae positive both at preliminary diagnosis and at discharge. The MLVA typing of the strains was consistent at two time points in the 49 patients. Among these 98 M. pneumoniae isolates collected from 49 pairs of patients, the most common type was 4-5-7-2 MLVA type (87.8%, 86/98), followed by the MLVA 4-5-7-3 (8.2%, 8/98) and 4-4-7-2 (4.1%, 4/98), respectively. The MLVA genotypes of the strains were consistent in those isolated from the same patient upon preliminary diagnosis or discharge.

3.5. Quantitative Culture Analysis of Viable M. pneumoniae of Clinical Samples

After excluding 2 pairs of samples with bacterial contamination (A26/B26 and A28/B28), CCU quantitative analysis was performed for the 47 pairs of M. pneumoniae culture positive samples. The content of viable M. pneumoniae in the preliminary diagnosis samples showed significant difference compared to that obtained upon discharge (10–104 CCU/mL vs. 10–102 CCU/mL, t = 2.980, P < 0.05). For the samples obtained from preliminary diagnosis, 6 samples showed a viable M. pneumoniae load of 10 CCU/mL, 20 showed a load of 102 CCU/mL, 18 showed a load of 103 CCU/mL, and 3 showed a load of 104 CCU/mL. At discharge, 30 showed a load of 10 CCU/mL, 12 showed a load of 102 CCU/mL, 1 showed a load of 103 CCU/mL, and 4 showed negative results. Thirty-seven cases showed smaller M. pneumoniae CCU value at discharge compared to that of the preliminary diagnosis. Eight cases showed consistent CCU value at two time points, and only two showed higher CCU values at discharge (Table 2 and Figure 2).

Table 2.

M. pneumoniae DNA quantitative analysis, number of viable bacteria, and culture duration of the 47 pairs of positive samples.

Preliminary diagnosis Discharge
Patient no. DNA load (copies/mL) Viable count (CCU/mL) TIIP (d) Patient no. DNA load (copies/mL) Viable count (CCU/mL) TIIP (d)
A002 5.96 × 103 10 20 B002 1.45 × 104 102 23
A003 5.28 × 102 10 19 B003 2.16 × 103 10 24
A005 1.76 × 104 103 17 B005 4.36 × 103 10 21
A006 2.79 × 103 10 17 B006 1.26 × 103 10 21
A008 6.94 × 103 102 19 B008 5.57 × 103 10 25
A009 1.97 × 103 102 21 B009 3.82 × 02 N N
A011 1.05 × 104 102 21 B011 3.83 × 02 N N
A012 9.60 × 103 103 14 B012 1.23 × 103 10 22
A016 2.45 × 104 103 8 B016 1.27 × 103 10 24
A021 5.75 × 103 102 17 B021 8.12 × 02 10 29
A024 3.32 × 103 102 24 B024 1.24 × 103 N N
A029 2.62 × 103 102 19 B029 4.11 × 103 10 25
A032 4.49 × 103 10 22 B032 1.11 × 103 10 28
A035 3.90 × 103 102 14 B035 1.82 × 103 N N
A037 5.30 × 103 102 12 B037 2.30 × 104 102 20
A040 4.45 × 103 102 18 B040 2.21 × 103 102 25
A041 9.56 × 103 103 18 B041 7.46 × 103 10 25
A042 6.69 × 103 103 15 B042 6.98 × 103 10 23
A043 3.51 × 103 103 18 B043 3.84 × 104 102 19
A045 7.67 × 103 102 14 B045 2.04 × 104 10 21
A047 6.95 × 103 103 17 B047 1.26 × 104 10 24
A051 8.74 × 103 102 18 B051 1.77 × 104 10 22
A053 8.91 × 103 102 13 B053 1.86 × 104 10 19
A055 1.75 × 104 103 12 B055 5.74 × 103 102 26
A056 1.56 × 104 103 14 B056 6.63 × 104 102 15
A058 4.75 × 104 104 18 B058 6.78 × 104 10 20
A059 4.81 × 104 103 8 B059 3.65 × 104 10 17
A060 9.52 × 103 102 13 B060 4.73 × 103 10 27
A061 3.01 × 104 103 10 B061 1.84 × 104 10 22
A062 5.22 × 103 102 16 B062 2.72 × 103 10 25
A065 2.04 × 104 103 13 B065 1.14 × 104 102 23
A068 8.46 × 103 103 16 B068 1.28 × 104 10 21
A069 1.50 × 103 102 21 B069 4.47 × 103 10 23
A070 7.85 × 103 10 16 B070 5.18 × 103 10 25
A072 1.94 × 104 103 16 B072 9.99 × 103 10 21
A073 1.11 × 104 102 19 B073 6.89 × 104 102 20
A074 1.36 × 104 103 14 B074 2.72 × 103 10 22
A075 1.95 × 105 104 9 B075 4.95 × 103 10 22
A076 9.32 × 103 102 13 B076 1.04 × 104 10 25
A080 1.12 × 104 103 10 B080 3.18 × 103 102 22
A081 3.93 × 103 10 26 B081 2.20 × 104 102 19
A086 2.13 × 103 102 25 B086 2.47 × 103 102 27
A087 2.49 × 104 103 8 B087 7.18 × 02 10 25
A088 8.03 × 103 102 18 B088 2.78 × 103 10 20
A089 7.68 × 104 104 9 B089 6.05 × 104 103 16
A090 1.67 × 105 103 7 B090 1.11 × 103 102 26
A091 3.30 × 104 102 12 B091 1.80 × 104 10 18
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N: negative.

Figure 2.

Figure 2

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Comparison of viable M. pneumoniae load and DNA quantitative analysis in samples that were negative upon preliminary diagnosis (a) and discharge (b).

3.6. TIIP

The shortest TIIP in the clinical samples was 7 days, and the latest TIIP was 30 days. Among the 92 cases, 80 showed a TIIP of 7–26 days for M. pneumoniae positivity at the preliminary diagnosis, while, at the discharge, 49 showed a TIIP of 16–30 days. Among the 47 pairs of M. pneumoniae positive samples, the TIIP of M. pneumoniae upon discharge was longer than that of the preliminary diagnosis in the samples of the same CCU. For the 8 patients with similar CCU value upon two time points (i.e., A03/B03, A06/B06, A32/B32, A37/B37, A40/B40, A70/B70, A73/B73, and A86/B86, Table 2), the TIIP of M. pneumoniae at discharge showed a 5.3-day delay compared to the preliminary diagnosis.

4. Discussion

In this study, 12 M. pneumoniae positive patients were IgM antibody negative, which then were IgM antibody positive about 4–6 days after preliminary diagnosis. This implied that the children were in an early stage of M. pneumoniae infection upon preliminary diagnosis, when serological test was not sufficient as there was no formation of IgM antibody or the titer of the antibody was not adequate. Compared with conventional serum IgM antibody determination, NAATs are superior in the early diagnosis of M. pneumoniae infection in order to improve the treatment efficiency and avoid antibiotics abuse.

Based on real-time PCR, Nilsson et al. [19] reported that about half of the subjects had detectable M. pneumoniae DNA in the oropharynx about 50 days, and even a longer duration of about 7 or more months. This indicated that M. pneumoniae DNA was available in oropharynx in a long term, which provided valuable information to the epidemiologic studies. The detection duration for DNA was more than 8 months in this report, which could not exclude the possibility of the M. pneumoniae reinfection. Moreover, DNA detection could not identify whether the target DNA fragment was from viable or nonviable organisms. Therefore, it is hard to discriminate the carrying status of the viable bacteria in each patient.

In this study, MLVA typing results were used to confirm infection of the same M. pneumoniae isolate. On this basis, possibilities of reinfection were excluded. The median hospitalization duration was 11 days, and the DNA positive rate at discharge was about 94.6%, which was similar with the previous study by Nilsson et al. [19] indicating up to 90% in the M. pneumoniae DNA positivity in throat about 10 days after infection. Thirty-three samples (40.2%) were positive for M. pneumoniae DNA at discharge; however, the culture results were negative. This implied a time delay in the clearance of DNA compared to the M. pneumoniae pathogen after treatment. These subjects were carriers of M. pneumoniae DNA other than viable isolates, who showed no infectious capability. In this study, freeze-thaw was performed once in the samples for the quantitative analysis. Among the M. pneumoniae positive samples, 4 cases showed M. pneumoniae negativity in the quantitative culture. This may be related to the potential effects of freeze-thaw on the viable bacteria number. Among the 47 patients that were M. pneumoniae positive at both preliminary diagnosis and discharge, 37 showed decrease in M. pneumoniae quantitative number at discharge (Table 2). Meanwhile, 43 patients were only M. pneumoniae positive at preliminary diagnosis (Figure 2). Taken together, 80 (88.9%) showed decrease of M. pneumoniae in number after treatment. Such trend could reflect the killing effects of antibiotics and immune clearance. The DNA used for the quantitative analysis was derived from viable M. pneumoniae and accumulated DNA from nonviable M. pneumoniae, which could not reflect the real carrying status of M. pneumoniae in each child at preliminary diagnosis or discharge. Therefore, the degradation and clearance of M. pneumoniae DNA are slow in vivo, and quantitative analysis is not adequate for the accurate determination.

The penicillin G and other bacteriostatic agents in the Mycoplasma selective medium can inhibit the majority of bacteria [25, 26]. Nevertheless, in few pharyngeal swabs, there were still bacteria resistant to penicillin, and there might be possibilities of bacterial contamination by the normal flora from the pharynx oralis. According to our experiences, the incidence of contamination by the bacteria in the swabs was in a range of 5% to 20%. In this study, significant differences were noticed in the bacterial contamination rate in the samples collected upon preliminary diagnosis and discharge (χ2 = 5.14, P < 0.05). This implied the clearance of penicillin-resistant bacteria in throat after macrolides antibiotics treatment. Indeed, it confirmed the side effects of antibiotics to the normal bacteria. On this basis, antibiotics were not recommended for the individuals with self-limited disease (e.g., mild M. pneumoniae infection) presenting mild symptoms [16, 27], in order to prevent the microbiota imbalance. For the analysis of CCU and TIIP of M. pneumoniae, obvious extension was observed in TIIP upon discharge compared with that of the preliminary diagnosis in the viable M. pneumoniae at the same CCU group (Table 3). Meanwhile, among the 8 cases with the same amount of M. pneumoniae, various delays were observed, and the extension of TIIP demonstrated growth inhibition of M. pneumoniae. Generally, in the absence of nonendogenous inhibiting agents, the effects of endogenous components on the culture of M. pneumoniae were nearly the same in a certain case. In this study, the endogenous components responsible for the delay of bacterial culture were likely to be the metabolites of macrolides antibiotics. This indicated that macrolides antibiotics and the metabolites showed inhibiting effects on M. pneumoniae.

Table 3.

Comparison of TIIP of M. pneumoniae culture quantitative analysis upon preliminary diagnosis and discharge.

Viable bacteria (CCU/mL) Positive sample TIIP TIIP, median TIIP, mean
Preliminary diagnosis Discharge Preliminary diagnosis Discharge Preliminary diagnosis Discharge Preliminary diagnosis Discharge
10 6 30 16–26 17–29 19.5 22.5 20 22.9
102 20 12 12–25 23–27 18 22 17.4 22.1
103 18 1 7–18 16 14 16 13.1 16
104 3 0 9–18 9 12
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—: not calculated.

In this study, we focused on the quantitative analysis of M. pneumoniae DNA and culture using same clinical samples. The clinical symptoms of the patients showed obvious remission after anti-infection therapy for M. pneumoniae, which was mainly characterized by M. pneumoniae clearance in about 40% of the patients after discharge, and decline of M. pneumoniae together with control of pathogenic bacteria in 60% of the patients. The clinical manifestations of patients with M. pneumoniae infection were featured by dry cough and small amount of sputum [27, 28]. Our data showed that 62 patients (67.4%) showed dry cough. For the patients in acute stage with typical symptoms and a large amount of M. pneumoniae, cough serves as an important source of infection. In spite of the fact that 60% of the patients were M. pneumoniae carriers of a small amount at discharge, these patients were symptom-free with very lower infectious capacity compared to that before treatment. Nevertheless, it is not sure whether these individuals are infectious or M. pneumoniae carriers, and then further studies are required.

There are limitations in our study. Firstly, it is not possible to follow up all the patients after discharge, and then the carrying status of the viable M. pneumoniae in the throat was not investigated in these patients. Secondly, we collected the samples using pharyngeal swabs, which may trigger bias in the amount of bacteria in the lower respiratory tract infection induced by M. pneumoniae. BALF samples may be ideal for this study. On this basis, further studies involving more accurate data are required.

In conclusion, we considered that DNA technique was rapid and effective for the qualitative diagnosis of M. pneumoniae at the early stage. However, it cannot be used to evaluate the prognosis of patients with M. pneumoniae infection, as well as the quantitative and qualitative analyses of M. pneumoniae. Qualitative culture was required to investigate the status of M. pneumoniae.

The numbers of specimens were arranged in an ascending order based on the number of viable bacteria.

Acknowledgments

This study was funded by the Major Infectious Diseases such as AIDS and Viral Hepatitis Prevention and Control Technology Major Projects (Grant nos. 2018ZX10712-001), the National Natural Science Foundation of China (Grant no. 81772154), and Non-profit Central Research Institute Fund of Chinese Academy of Medical Sciences (Grant no. 2018RC310027).

Data Availability

All the data were available upon appropriate request.

Disclosure

Fei Zhao, Xuemei Guan, and Jing Li contributed equally to this work.

Conflicts of Interest

The authors declare that there are no conflicts of interest regarding the publication of this paper.

Authors' Contributions

ZF wrote the manuscript. ZJZ revised the manuscript. GXM, LJ, and LLY did the data analysis. GJ, HLH, and MFL did the data collection.

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Data Availability Statement

All the data were available upon appropriate request.

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