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JoVE Journal Immunology and Infection

Immunology and Infection

Rapid Detection of Bacterial Pathogens Causing Lower Respiratory Tract Infections via Microfluidic-Chip-Based Loop-Mediated Isothermal Amplification

Published: March 29, 2024 doi: 10.3791/66677
*1,2, *1,3, *4, 1, 1, 2, 2, 2, 1
1Laboratory Medicine, Guangdong Provincial People’s Hospital (Guangdong Academy of Medical Sciences), Southern Medical University, 2Department of Laboratory Medicine, Shengli Oilfield Central Hospital, 3Guangdong Cardiovascular Institute, Guangdong Provincial People’s Hospital (Guangdong Academy of Medical Sciences), Southern Medical University, 4Dermatology Hospital, Southern Medical University
* These authors contributed equally

Abstract

Respiratory tract infections (RTIs) are among the most common problems in clinical settings. Rapid and accurate identification of bacterial pathogens will provide practical guidelines for managing and treating RTIs. This study describes a method for rapidly detecting bacterial pathogens that cause respiratory tract infections via multi-channel loop-mediated isothermal amplification (LAMP). LAMP is a sensitive and specific diagnostic tool that rapidly detects bacterial nucleic acids with high accuracy and reliability. The proposed method offers a significant advantage over traditional bacterial culturing methods, which are time-consuming and often require greater sensitivity for detecting low levels of bacterial nucleic acids. This article presents representative results of K. pneumoniae infection and its multiple co-infections using LAMP to detect samples (sputum, bronchial lavage fluid, and alveolar lavage fluid) from the lower respiratory tract. In summary, the multi-channel LAMP method provides a rapid and efficient means of identifying single and multiple bacterial pathogens in clinical samples, which can help prevent the spread of bacterial pathogens and aid in the appropriate treatment of RTIs.

Introduction

Respiratory tract infections (RTIs) caused by bacterial pathogens primarily contribute to morbidity and mortality worldwide1. It is defined as any upper or lower respiratory symptoms accompanied by fever lasting 2-3 days. While upper respiratory infection is more common than lower respiratory infection, chronic and recurrent respiratory tract infections are also common clinical conditions, posing great risks to individuals and placing a significant burden on healthcare systems2. Common bacterial pathogens of RTIs include Streptococcus pneumoniae3, Haemophilus influenzae4, Staphylococcus aureus, Escherichia coli, Klebsiella pneumoniae, Stenotrophomonas maltophilia, among others. These pathogenic bacteria usually colonize the mucosal surfaces of the host's nasopharynx and upper respiratory tract, causing typical symptoms of RTIs such as sore throat and bronchitis. They cause pneumonia when they spread from the upper respiratory tract to sterile areas of the lower respiratory tract and may spread from person to person through the respiratory tract5. In severe cases, they can also lead to invasive bacterial diseases, especially bacteremic pneumonia, meningitis, and sepsis, which are leading causes of morbidity and mortality in people of all age groups worldwide.

Traditional tests for RTIs involve microbiological culture using throat swabs and sputum respiratory samples6. Additionally, serological tests such as enzyme-linked immunosorbent assay (ELISA) detect antibodies or antigens in serum, while agglutination tests observe the agglutination reaction of antibodies and antigens to detect infection7. Microbial culture is considered the gold standard for diagnosing RTIs, but its low culture positivity rate, poor reliability, and long detection cycle limit diagnostic efficiency8. In reality, rapid and accurate diagnosis of RTIs is crucial for precise eradication of the bacterial pathogen. Quick and effective detection methods can help reduce the transmission rate of pathogens, shorten the duration of infection, and decrease unnecessary antibiotic use9,10. Molecular biology-based methods significantly expedite detection, such as polymerase chain reaction (PCR), which amplifies a target gene's DNA sequence to detect pathogens. However, traditional PCR necessitates complex temperature cycling equipment, which is cumbersome and time-consuming. Furthermore, every DNA amplification using PCR (except real-time PCR) concludes with electrophoretic separation of the product, which also takes time. Visualization of the product requires dyes, many of which are mutagenic or carcinogenic. Therefore, it is imperative to continuously develop new methods and technologies for diagnosing RTI bacterial pathogens.

Loop-Mediated Isothermal Amplification (LAMP) is a novel and emerging molecular technology initially developed by Notomi et al. in 200011. LAMP can amplify DNA under stable isothermal conditions without complex temperature cycling equipment, which makes it suitable for rapid detection and reduces equipment complexity and cost12. LAMP can detect low concentrations of target DNA with high sensitivity13. It uses multiple specific primers to improve selectivity for target sequences and reduce the possibility of false positives14. LAMP is gradually being widely used in clinical laboratories due to its ease, speed, and intuitive operation, even for detecting RTIs. In this study, we investigated the effectiveness of LAMP in detecting lower RTIs in clinical samples (sputum, bronchial lavage fluid, and alveolar lavage fluid), as shown in Figure 1. It is evident that LAMP offers advantages such as speed, sensitivity, and ease of use over traditional tests in lower RTI detection, making it a promising application.

Figure 1
Figure 1: Schematic illustration of the LAMP detection method. Please click here to view a larger version of this figure.

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Protocol

All samples for this study were evaluated and approved by the Ethics Review Committee of Guangdong Provincial People's Hospital (Approval Number: KY2023-1114-01). All participants signed written informed consent before the experiments. The reagents and equipment used for the study are listed in the Table of Materials. The abbreviations used in the protocol are listed in Supplementary Table 1.

1. Collection of clinical samples from the lower respiratory tract

  1. Sputum collection
    1. Cleanse the oral cavity and teeth with clean water, ensuring denture removal if applicable. Cough forcefully to expel deep respiratory sputum into a sputum container (minimum 0.6 mL).
    2. Avoid contamination with saliva or nasal discharge. If coughing is difficult, administer inhalation of a 100 g/L NaCl solution at 45 °C to facilitate expectoration. Transfer the specimen to a sterile, sealable container.
      NOTE: Ensure the sputum samples are collected in the morning and before any antibacterial drug use.
  2. Bronchial lavage fluid (BLF)
    1. Insert the collector head into the trachea from the nostril or tracheostomy site (approximately 30 cm deep). Inject 5 mL of saline, establish negative pressure, rotate the collector head, and slowly withdraw.
    2. Collect the extracted mucus and rinse the collector once with a sampling solution (physiological saline or sterile water for injection). Alternatively, connect a pediatric urinary catheter to a 50 mL syringe as a substitute for collection.
  3. Alveolar lavage fluid (ALF)
    1. Identify the lesion location through chest imaging examinations. Select the most significant or rapidly progressing area for lavage.
    2. Inject 1-2 mL of 2% lidocaine into the bronchial segment through the biopsy channel during lavage, providing local anesthesia for the lavaged lung segment15. For patients under intravenous general anesthesia who still exhibit strong airway reactions, inject 1-2 mL of 2% lidocaine.
    3. After local anesthesia, insert a fiberoptic bronchoscope through the mouth or nose, passing through the pharynx into the bronchus of the right middle lobe or the lingual segment of the left lung. Place its tip at the opening of the bronchial branch and slowly introduce sterile physiological saline.
    4. Administer 30-50 mL saline per session, with 100-250 mL volume (max. 300 mL). Collect the extracted mucus in a sealed sterile container.

2. DNA extraction

  1. Based on the viscosity of lower respiratory tract samples, add an appropriate amount of 10% NaOH. For samples with low viscosity, add 2-3 times the volume of the sample of liquefying solution. For samples with moderate viscosity, add 5-6 times the volume of the sample of liquefying solution. For samples with high viscosity, add 8-10 times the volume of the sample of liquefying solution.
    1. Adjust the volume of 10% NaOH according to the sample viscosity. Disperse the samples as uniformly as possible using a vortex mixer for 15 s and incubate at 37 °C for 30 min for liquefaction.
      NOTE: For thicker samples, increase the volume of NaOH or extend the liquefaction time. The liquefaction quality of samples directly influences the subsequent extraction efficiency. Ideally, liquefied samples should exhibit a consistent, non-sticky consistency.
  2. Pipette 1 mL of the liquefied sample into a 1.5 mL centrifuge tube. Centrifuge at a speed of 15,777 × g for 5 min at 2-6 °C, then use a pipette to remove and discard the supernatant.
    NOTE: When aspirating the sample, avoid drawing impurities from the bottom of the tube; if there are many impurities, the sample can be centrifuged at 1,753-2,739 × g for 1 min before aspiration.
  3. Add 1 mL of washing solution to the centrifuge tube and vortex to lift the precipitate from the bottom of the tube. There is no need to disperse it completely.
    1. Centrifuge the solution at 15,777 × g for 5 min, discard the supernatant, and try not to touch the precipitate.
      NOTE: Ensure thorough removal of the washing solution to avoid affecting subsequent amplification.
  4. Add 100 µL of nucleic acid extraction solution to the centrifuge tube. Use a pipette to aspirate and mix the precipitate thoroughly. Transfer the liquid and precipitate together into a nucleic acid extraction tube. The composition of the nucleic acid extraction solution is presented in Table 1.
  5. Place the nucleic acid extraction tubes in a vortex mixer and vortex at medium speed for at least 5 min. After vortexing, transfer the nucleic acid extraction tubes to a metal bath with a constant temperature and heat at 100 °C for 5 min.
  6. Centrifuge at 15,777 × g at 2-6 °C for 5 min and set aside.
    NOTE: If the PCR amplification reaction is performed within 24 h, the nucleic acid can be stored at 4 °C. After the amplification, store the nucleic acid at -20 °C. For long-term storage (beyond 24 h), store the nucleic acid at -20 °C. When ready to use again, thaw the sample naturally, vortex to mix, heat in a 95 °C water bath for 5 min, centrifuge at 10,956 × g for 1 min, and use the supernatant for PCR amplification.
Solution Components Number Specification
Washing Solution 10 mM EDTA 1 bottle 24 mL/bottle
Nucleic Acid Extraction Reagent 10mM Tris-HCl, 1mM EDTA, Nucleic acid preservatives 2 tubes 1.2 mL/bottle
Nucleic Acid Extraction Tube Glass beads 1 bag 24 bottles/bag

Table 1: Composition of nucleic acid extraction reagent.

3. Loop-mediated isothermal amplification and microfluid chip

  1. Reagent and microfluidic chip
    1. Conduct isothermal amplification reactions on a microfluidic disk-shaped chip (see Table of Materials). Carry out the constant-temperature amplification at 65 °C.
    2. Perform real-time fluorescence analysis using a fluorescent dye incorporation method14 on the constant-temperature amplification microfluidic chip nucleic acid analyzer. Observe an S-shaped amplification curve for positive samples using a polymerase with strand displacement functionality.
  2. Loop-mediated isothermal amplification
    1. Target six sequence regions with four specific primers, including two inner primers and two outer primers (provided with the LAMP kit).
      NOTE: DNA is continuously replicated and amplified at a constant temperature using a DNA polymerase with strand displacement functionality. The reaction process involves the dumbbell-shaped template synthesis stage, cycling amplification stage, elongation, and recycling stage, ultimately forming a mixture of DNA fragments with stem-loop and cauliflower-like structures. Refer to the kit instructions for detailed information (Supplementary File 1).
    2. Add two-loop primers to the reaction system to enhance reaction efficiency, which binds to the stem-loop structures, initiating strand displacement synthesis and cyclic replication. The composition of the nucleic acid detection kit for respiratory tract pathogens is presented in Table 2.
      NOTE: The reagent kit utilizes the LAMP method. The principle is based on the dynamic equilibrium of DNA at around 65 °C, where any primer extending through base pairing at the complementary site of double-stranded DNA causes the other strand to dissociate, forming a single strand.
  3. Microfluidic chip
    NOTE: Each microfluidic chip (see Table of Materials) is equipped with 24 reaction wells numbered counterclockwise, with the inlet and outlet for well 1 corresponding to the reaction well 1 (Figure 2). A specific set of primers for amplification and detection of a particular nucleic acid target sequence is embedded and fixed in each reaction well.
    1. Mix the sample DNA with the amplification reagent. Inject the mixture into the chip and distribute it to each reaction well centrifuge at 1,000 × g for 30 s at room temperature.
      NOTE: Independent isothermal amplification reactions and real-time fluorescence detection co-occur in each reaction well on the chip. If an S-shaped amplification curve is detected in a particular reaction well, the corresponding detection index for that well is positive.
Components Composition Number
Chip Primers 12 places
Sealing Film / 1 sheet
Isothermal Amplification Reagent Fluorescent dye, Enzyme 270 µL/tube
Positive Control Escherichia coli Genomic DNA 160 µL/tube

Table 2: Composition of nucleic acid detection kit for respiratory tract pathogens.

Figure 2
Figure 2: Disc chip structure diagram. The reaction wells are sequentially numbered counterclockwise, where the inlet/outlet port 1 corresponds to the reaction well number 1. Reaction wells 1, 4, 7, 10, 13, 16, 19, 22, and 24 are negative controls. Reaction well 6 is a positive control (E. coli). The reaction well 12 is an internal positive control, and reaction well 23 is an external positive control. Reaction well 2 detects spn. Reaction well 3 detects sau. The reaction well 5 detects MRSA. The reaction well 8 detects kpn. The reaction well 9 detects pae. The reaction well 11 detects aba. The reaction well 14 detects sma. The reaction well 15 detects hin. Please see Table 5 for sample details. Please click here to view a larger version of this figure.

4. Sample preparation and bacterial detection

  1. Prepare the isothermal amplification reaction system
    1. Take the isothermal amplification reagent from the kit and allow it to thaw at room temperature fully. Gently shake to mix thoroughly and centrifuge briefly to collect at the bottom of the tube.
    2. In the reagent storage and preparation area, pipette 20 µL of the isothermal amplification reagent into a prepared 200 µL centrifuge tube. Cover the tube and move it to the specimen preparation area with one centrifuge tube per sample.
    3. In the specimen preparation area, add 34.5 µL of the target nucleic acid sample. Shake gently to mix thoroughly and centrifuge briefly to collect at the bottom of the tube. The total volume of each nucleic acid amplification reaction system is 54.5 µL (Table 3).
  2. Chip loading procedure
    1. On the chip packaging, label the sample number. Open the microfluidic chip with the packaging label facing up.
    2. Place the chip with the inlet and outlet ports facing upwards. Using a pipette, draw 50 µL of the prepared amplification reaction system and add it to the main channel of the chip through the inlet port. Stop adding when the main channel is filled, and quickly wipe off any excess liquid around the inlet and outlet ports with lint-free tissue.
    3. Use tweezers to pick up one sealing film and cover it over the inlet and outlet ports. Press a clean pipette tip onto the sealing film in one direction. Ensure a tight seal.
  3. qPCR reaction
    1. After the light source of the nucleic acid analyzer has completed preheating, click on the Open Tray button. Place the chip with the front side up on the tray, ensuring that the locating small cylinder emerges from the center gap of the chip to secure it. Align the center positioning device in the tray with the large central hole in the chip.
    2. Click on the Close Tray button to insert the chip into the nucleic acid analyzer.
    3. In the Sample Information area on the detection interface, enter the information for testing the sample. Sample number, chip number, and sample type are mandatory; others are optional.
    4. Click on the Start Detection button in the operation area to initiate the sample detection. The instrument will conduct sample testing according to the preset program.
      NOTE: After the completion of detection, the accompanying software of the device will automatically conduct data analysis. Simultaneously, the nucleic acid analyzer will initiate an automatic cooling process. Once the temperature drops to 37 °C, the instrument automatically opens the tray and ejects the chip for retrieval. The results will be interpreted automatically by the system (Table 4).
  4. Quality control standards
    1. One positive quality control and nine negative quality controls are enclosed in each chip in this reagent kit. Ensure that the detection results for the positive quality control is positive, and simultaneously, the results for all nine negative quality controls are negative.
      NOTE: The results are displayed on the right side of the image stating "Quality Control Results: Experiment Normal (Positive Normal, Negative Normal)," indicating that the test results are valid. Retest is required if any result is incorrect and the sample test result is deemed invalid. One positive internal control using human-specific primers is enclosed in the chip, the result of which is positive for clinical sample testing while being negative if the sample has a low human genomic DNA content, indicating a lower cell count. Recollect and retest samples in such cases.
  5. Results analysis
    1. After completion of the detection, utilize the second-derivative maximum method combined with commercially protected algorithms in the software to calculate the first inflection point of the S-shaped amplification curve during the rapid amplification phase. Details are described in the "Principles of the Test" part of Respiratory Pathogens Nucleic Acid Detection Kit Instructions (Supplementary File 1).
      NOTE: The TP value is the time difference between the inflection point and the origin. The result is interpreted based on the TP and positive judgment values. If the TP value for a detection index is less than or equal to the positive judgment value for that index, it is interpreted as positive. If the TP value exceeds the positive judgment value, it is interpreted as negative, according to the criteria for "positive decision value" in the instructions. The "Fluorescence Curve Area" displays the normalized curve, and the "Detection Result" area shows the quality control and detection results for each parameter (Table 5).
Reactant Volume (µl)
Isothermal Amplification Reagent 20
Template DNA 34.5

Table 3: Isothermal amplification reaction system.

Step One Two
Temperature (°C) 37 65
Time (min) 3 47

Table 4: Nucleic acid amplification reaction program.

Indicator Name Positive Control Value
Streptococcus pneumoniae (sp) 30
Staphylococcus aureus (sau) 34
Methicillin-resistant Staphylococcus aureus  (mrsa) 22
Klebsiella pneumoniae (kpn) 29
Pseudomonas aeruginosa (pae) 36
Acinetobacter baumannii (aba) 36
Stenotrophomonas maltophilia (sma) 27
Haemophilus influenzae (hin) 36

Table 5: Positive control value for infection indicator.

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Representative Results

This experiment employs isothermal amplification technology, conducting reactions on a microfluidic disc chip. The reaction occurs on a microfluidic chip nucleic acid analyzer, employing a fluorescence dye insertion method. The isothermal reaction is performed at a constant temperature of 65 °C, and real-time fluorescence analysis is carried out simultaneously. Positive samples undergo amplification under the action of polymerase with chain displacement functionality, resulting in an S-shaped amplification curve. This one-step process completes the amplification and detection of the target gene. This study selected 7 samples with different experimental outcomes to demonstrate the reliability of the experimental design. The capital letter S stands for a sample. S1 is a sample infected with a single strain of K. pneumoniae. S2 to S7 are samples with polymicrobial infections, all infected with K. pneumoniae. For effective detection results, interpretation can be made through the normalized fluorescence curves displayed in the images. A positive indicator is represented by an amplification curve exhibiting an S-shape, while a horizontal line represents a negative indicator (Figure 3).

Figure 3
Figure 3: Representative nucleic acid amplification results via LAMP. The capital letter S stands for sample. S1 is a sample infected with a single strain of kpn. S2 to S7 are samples with polymicrobial infections, all infected with kpn. S2 represents a sample infected with kpn and sma. S3 denotes a sample concurrently infected with kpn, sau, and MRSA. S4 signifies a sample concurrently infected with kpn, sau, MRSA, and aba. S5 indicates a sample concurrently infected with kpn, sma, sau, MRSA, and aba. S6 denotes a sample concurrently infected with kpn, sma, pae, sau, MRSA, and aba. S7 represents a sample concurrently infected with kpn, sma, pae, sau, MRSA, aba, and E. coli. Please see Table 5 for sample details. Please click here to view a larger version of this figure.

This reagent kit utilizes the ROC method to calculate positive threshold values for eight test indicators. When the TP value of a detection indicator is less than or equal to its corresponding positive threshold value, it is interpreted as positive. Conversely, when the TP value of a detection indicator is greater than its positive threshold value, it is interpreted as negative. The positive threshold values for each indicator are detailed in Table 5. The true positive TP values we detected for the 7 samples with different experimental outcomes are shown in Table 6.

SAMPLE kpn sma pae sau mrsa hin aba eco
TP (+/-) TP (+/-) TP (+/-) TP (+/-) TP (+/-) TP (+/-) TP (+/-) TP (+/-)
S1 19.68 (+) U (-) U (-) U (-) U (-) U (-) U (-) U (-)
S2 17.73 (+) 18.30 (+) U (-) U (-) U (-) U (-) U (-) U (-)
S3 16.73 (+) U (-) U (-) 18.05 (+) 12.18 (+) U (-) U (-) U (-)
S4 21.66 (+) U (-) U (-) 27.07 (+) 19.61 (+) U (-) 18.29 (+) U (-)
S5 16.16 (+) 20.85 (+) U (-) 23.80 (+) 17.13 (+) U (-) 15.22 (+) U (-)
S6 11.20 (+) 16.79(+) 17.18(+) 23.09 (+) 16.14 (+) U (-) 14.28 (+) U (-)
S7 14.69 (+) 24.84(+) 19.70(+) 24.07(+) 14.16 (+) - (+) 15.23 (+) 20.12 (+)
Each Sample+/-, qualitative result;
 +, positive result; -, negative result. 

Table 6: Table of TP values for detection after infection.

Supplementary Table 1: List of abbreviations. Please click here to download this File.

Supplementary File 1: Respiratory pathogens nucleic acid detection kit instructions. Please click here to download this File.

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Discussion

Respiratory tract infections are prevalent hospital-associated infections, imposing severe consequences on patients and escalating mortality rates16. Timely and accurately identifying potential pathogens followed by effective antibiotics is the key to successful treatment and improving prognosis, particularly given the limitations inherent in traditional culture methods17. In this study, we used a LAMP-based method to determine single or multiple infections for fast and precise detection of RTIs. This quick detection system is established by combining LAMP technology with microfluidic technology. The nucleic acid from clinical samples, such as sputum, BLF, and ALF, can be extracted quickly. This extracted material facilitates the rapid and precise detection of bacterial pathogens, guiding clinical practices for improved control and treatment of RTIs.

Previous studies have shown that compared to culture-based methods and polymerase chain reaction, LAMP results achieved 100% sensitivity, specificity, and no cross-reaction with other bacteria in pure cultures and blood samples18. LAMP assays can also detect pathogens directly from biological fluids, such as blood, pleural and peritoneal fluid, and cerebrospinal fluid19. It has been previously demonstrated that exogenous DNA and inhibitors may significantly reduce the sensitivity of PCR, and for LAMP assays, purification of DNA from clinical specimens is not required20. This technique utilizes yeast genes and primers during the amplification process to assess the normalcy of the amplification, thereby determining the qualification of external control quality control. Internal controls, employing primers from human genes, determine the normalcy of sampling, nucleic acid extraction, and amplification processes. Simultaneous utilization of internal and external controls ensures the reliability of the results. At the same time, multiple positive and negative control wells are also set up, which greatly ensures the accuracy of the test. LAMP microfluidic chip has capabilities similar to qPCR in detecting clinical specimens. It has the characteristics of high sensitivity and strong detection ability, providing a reliable basis for rapid clinical detection and precise treatment21. Microbial culture takes 3-5 days or even longer, and some pathogens, such as Chlamydia pneumoniae and Legionella pneumophila, cannot be cultured. In contrast, LAMP detects multiple bacterial pathogens, even the unculturable, in less than 3 h, significantly increasing detection speed.

It can also perform multiple detections. The LAMP microfluidic chip is divided into various reaction units that detect multiple pathogens in parallel, ensuring the independence of each reaction and the accuracy of the results22,23. The data from the China Network Antibacterial Surveillance Center showed that the prevalence of K. pneumoniae ranked first among the bacterial isolates from respiratory specimens in 202215. Among the respiratory samples collected by Guangdong Provincial People's Hospital in 2022, the positive rate of K. pneumoniae tested by LAMP was 18.6%, which is also one of the bacteria with the highest prevalence. In all K. pneumoniae-positive samples, 30.6% were infections caused solely by K. pneumoniae, and 29.7% were infections where K. pneumoniae coexisted with other bacterial species. Additionally, there were triple infections (23.9%) and quadruple infections (10.5%) involving K. pneumoniae infection, constituting the majority in KP-positive samples, approximately 95%. There were very few cases of quintuple and sextuple infections, and as of now, infections beyond sextuple have not been detected. The results demonstrate six representative scenarios, each representing the detection results of infections caused by K. pneumoniae alone or coexisting with 1-5 other bacterial species.

In addition, the LAMP chip technology used in this study can also detect bacterial resistance. It detects methicillin-resistant MRSA via the mecA gene. When the wells representing Staphylococcus aureus and the wells for the mecA gene are positive, they represent a methicillin-MRSA infection. Researchers are continuously exploring methods for simultaneously rapidly detecting pathogens and antibiotic resistance traits. For example, a rapid diagnostic method for Helicobacter pylori infection and antibiotic resistance is based on quantitative polymerase chain reaction (qPCR)24. Another approach involves quickly predicting multidrug-resistant K. pneumoniae through deep learning analysis of surface-enhanced Raman scattering (SERS) spectra25 and a method for detecting K. pneumoniae and carbapenemase genes using SERS spectra26. Additionally, there is a classification and prediction method for different multi-locus sequence typing (MLST) profiles of K. pneumoniae strains based on SERS spectra analysis27. We will also subsequently develop sensitive and accurate detection of K. pneumoniae and carbapenemase genes, with performance comparable to gold-standard clinical methods that are time-consuming or based on expensive specialized instruments. Moreover, the ideal diagnostic approach is fast, accurate, cost-effective, and user-friendly18. A study estimating the cost of reagents for current diagnostic technologies showed that sample testing based on PCR technology costs up to US$6.4-7.7, compared with only US$0.71-2 for LAMP technology28.

The multi-channel loop-mediated isothermal amplification (LAMP) method, while offering significant advantages for the rapid detection of bacterial pathogens in respiratory tract infections, has its limitations. The high sensitivity of LAMP poses a risk of cross-contamination, where minimal DNA contamination can lead to false-positive results29; thus, stringent sample handling and procedural protocols are necessary to mitigate this risk. Despite the method's simplicity, the interpretation of results requires specific expertise and experience to avoid misinterpretation or diagnostic errors, emphasizing the need for well-trained personnel. Recognizing these limitations is essential for the effective application and further development of the LAMP method in the field of clinical diagnostics. Taken together, the LAMP method combined with a microfluidic chip can rapidly detect various bacterial pathogens in parallel. It has the advantages of high sensitivity and strong specificity and the features of low cost, rapidness, and convenience. It shows considerable practical significance for preventing and controlling RTIs caused by pathogenic infections in clinical settings. The significant feature of the LAMP test proposed in this study is that it is easy for laboratory staff to master, which is of great help to primary hospitals, disease prevention, control centers, and inspection and quarantine departments. In summary, the LAMP microfluidic chip system is a powerful detection tool in clinical laboratories, which can solve the high expenditure and low turn-around-time challenges in clinical infection diagnosis and has significant application values in clinical settings.

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Disclosures

The authors declare no conflict of interest.

Acknowledgments

We greatly appreciated the financial support provided by the Guangdong Basic and Applied Basic Research Foundation (Grant No. 2022A1515220023) and the Research Foundation for Advanced Talents of Guandong Provincial People's Hospital (Grant No. KY012023293).

Materials

Name Company Catalog Number Comments
Bath Incubator(MK2000-2) ALLSHENG Provide a constant temperature environment
Bronchial lavage fluid collector head TIANPINGHUACHANG SEDA 20172081375 Collecting bronchoalveolar lavage fluid
Fiberoptic bronchoscope OLYMPUS SEDA 20153062703 A flexible bronchoscope equipped with a fiberoptic light source and camera, to visually examine the airways and structures within the lungs. Assist in collecting bronchoalveolar lavage
HR1500-Equation 1B2 Haier SEDA 20183541642 Biosafety cabinet
NAOH MACKLIN S817977 Liquefy viscous lower respiratory tract sample
Nucleic acid detection kit for respiratory tract pathogens Capitalbio Technology SEDA 20173401346 Testing for bacteria infection
Nucleic acid extraction reagent Capitalbio Technology SEDA 20160034 For DNA extraction
RTisochip-W Capitalbio Technology SEDA 20193220539 Loop-mediated Isothermal Amplification
THERMO ST16R Thermo Fisher Scientific SEDA 20180585 Centrifuge the residual liquid off the wall of the tube.
Vortex mixer VM-5005 JOANLAB For mixing reagent

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References

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Respiratory tract infection Bacterial pathogen Klebsiella pneumoniae Sputum Loop-mediated isothermal amplification
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Lai, J. X., Qin, Y. R., Liao, Y. W., More

Lai, J. X., Qin, Y. R., Liao, Y. W., Si, Y. T., Yuan, Q., Huang, S. M., Tang, Y. R., Wang, J. L., Wang, L. Rapid Detection of Bacterial Pathogens Causing Lower Respiratory Tract Infections via Microfluidic-Chip-Based Loop-Mediated Isothermal Amplification. J. Vis. Exp. (205), e66677, doi:10.3791/66677 (2024).

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