Proof of Concept for a Portable Platform for Molecular Diagnosis of Tropical Diseases

Rampazzo, Rita de Cássia Pontello; Graziani, Ana Cláudia; Leite, Keren K.; Surdi, Jhully Anni; Biondo, Cheysa A.; Costa, Maykon L.N.; Jacomasso, Thiago; Cereda, Marco; Fazio, Marco; Bianchessi, M; Moreira, Otacílio C.; Britto, Constança; Costa, Joana D'Arc Neves; Góes, Viviane Monteiro; Silva, Alexandre J. da; Krieger, Marco Aurélio; Costa, Alexandre Dias Tavares

doi:10.1016/j.jmoldx.2019.04.008

Cited by 23 publications

(24 citation statements)

References 49 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…The low number of samples analyzed in the present study limits our ability to draw definitive conclusions, but the results obtained with the optimized protocol showed good agreement with results obtained by reference diagnosis methods such as culture or other molecular tests, providing the basis for future studies. The ready-to-use reactions performed similarly to the conventional ones, exhibiting similar lower detection limits, as previously shown for detection of T. cruzi or Plasmodium spp DNA [12]. After evaluation of larger cohorts, we suggest that the ready-to-use reactions could be implemented in places with unreliable power supply, as in urban suburbs and rural areas of high TB burden countries of Brazil, India, Indonesia, China, Philippines and Pakistan.…”

Section: Plos Onesupporting

confidence: 72%

“…An overview of the full procedure is outlined in Fig 3, showing a direct comparison to the general workflow of commercially available spin-column extraction kits. Although the ASSURED requirements have been met to a large extent in platforms such as GeneXpert Ultra or BioFire, the Q3-Plus system shows some advantages over both the aforementioned instruments and the standard benchtop ABI7500 in terms of equipment and reaction costs, reaction volume, user friendly interface, fast temperature ramping, and shorter total reaction time [12,20]. Some of these features will be further discussed below.…”

Section: Discussionmentioning

confidence: 99%

“…all qPCR reagents (enzymes, buffers, oligonucleotides, dNTPs, etc.) and 5 μL of in substitution for molecular-grade water in [12,[17][18][19]. The gelification solution contains three classes of components, each with specific functions within the mixture and the process: (i) trehalose and melezitose (400 mg/mL each), to protect the biomolecules from the desiccation process by stabilizing and reducing the activity of water in the solution; (ii) lysine (0.75 mg/mL), a free radical scavenger which inhibits oxidizing reactions between carbonyl or carboxyl groups and the biomolecule's amino or phosphate groups; and (iii) glycogen (200 mg/mL), an inert polymer which creates a broader protective matrix.…”

Section: Gelification Of Qpcr Reagentsmentioning

confidence: 99%

“…The gelification solution contains three classes of components, each with specific functions within the mixture and the process: (i) trehalose and melezitose (400 mg/mL each), to protect the biomolecules from the desiccation process by stabilizing and reducing the activity of water in the solution; (ii) lysine (0.75 mg/mL), a free radical scavenger which inhibits oxidizing reactions between carbonyl or carboxyl groups and the biomolecule's amino or phosphate groups; and (iii) glycogen (200 mg/mL), an inert polymer which creates a broader protective matrix. These components define a sol-gel mixture that prevent the loss of the tertiary or quaternary structure during the desiccation process, thus helping maintaining the biomolecules' activity upon rehydration [12,17]. The final concentration of each component of the gelification mixture used in this study was trehalose 160 mg/mL, melezitose 80 mg/mL, glycogen 40 mg/mL and lysine 0.15 mg/mL.…”

Section: Gelification Of Qpcr Reagentsmentioning

confidence: 99%

“…A rapid, simple, efficient, less expensive and ideally equipment-free sample preparation would not only bring down the cost of molecular assays but also mitigate the challenge of access to low-resource settings [9,10]. Furthermore, the reagents used in molecular assays require special storage and transportation, which further increase their costs [11,12]. Largely, the successful integration of sample preparation with ready-to-use reagents and portable qPCR systems would solve the main hurdles in point of care testing [9,10,13].…”

Section: Introductionmentioning

confidence: 99%

See 4 more Smart Citations

Demonstration of a fast and easy sample-to-answer protocol for tuberculosis screening in point-of-care settings: A proof of concept study

et al. 2020

Self Cite

View full text Add to dashboard Cite

We sought to develop a smooth and low cost sample preparation and DNA extraction protocol, streamlined with a ready-to-use qPCR in a portable instrument to overcome some of the existing hurdles. Several solutions were evaluated as to their ability to liquefy a mucin-based matrix. Each liquefied matrix, supplemented with either Mycobacterium tuberculosis (MTB) H37Rv strain DNA or intact cells, was aliquoted onto a filter paper embedded with solubilizing agents, and was subsequently dried up. Most of the nucleic acids, including genomic DNA from the bacilli and the host, binds to the filter paper. Next, several protocols were evaluated to elute the DNA from the paper, using qPCR to detect the insertion sequence IS6110, a M. tuberculosis complex genomic marker. The limit of detection (LOD) of the best protocol was then evaluated using parallel seeding and colony counting. The protocol was also evaluated using seventeen sputum samples, previously characterized by the GeneXpert or culture. Two instruments (the ABI7500 Standard and the Q3-Plus system) and two reagents storage formats (frozen or ready-to-use) were evaluated. Solutions containing guanidine isothiocyanate exerted the best liquefying effect on the mucin-based matrix extracted from one 6-mm punches, followed by a brief incubation at 95°C. The resulting DNA contained impurities, but a simple 1:10 dilution elicited the detection of MTB and human genomic targets. The described protocol presented an apparent LOD of 02 CFU/mL of MTB. Challenging the protocol with previously characterized samples showed substantial agreement with GeneXpert MTB/RIF results (sensitivity of 90%, agreement of 88.9%, kappa coefficient of 0.77), and moderate agreement with culture results (sensitivity of 100%, agreement of 78.9%, kappa coefficient of 0.58). This work presents a sensitive proof–of-concept protocol for sputum liquefaction and decontamination followed by a simple DNA extraction procedure, in which the extraction steps are streamlined with a ready-to-use qPCR in a portable instrument that can be employed in low infrastructure settings.

show abstract

Section: Plos Onesupporting

confidence: 72%

Section: Discussionmentioning

confidence: 99%

Section: Gelification Of Qpcr Reagentsmentioning

confidence: 99%

Section: Gelification Of Qpcr Reagentsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 3 more Smart Citations

Demonstration of a fast and easy sample-to-answer protocol for tuberculosis screening in point-of-care settings: A proof of concept study

et al. 2020

Self Cite

View full text Add to dashboard Cite

show abstract

Diagnosis of Malaria Parasites Plasmodium spp. in Endemic Areas: Current Strategies for an Ancient Disease

Gitta¹,

Kilian

2019

BioEssays

View full text Add to dashboard Cite

Fast and effective detection of the causative agent of malaria in humans, protozoan Plasmodium parasites, is of crucial importance for increasing the effectiveness of treatment and to control a devastating disease that affects millions of people living in endemic areas. The microscopic examination of Giemsa‐stained blood films still remains the gold‐standard in Plasmodium detection today. However, there is a high demand for alternative diagnostic methods that are simple, fast, highly sensitive, ideally do not rely on blood‐drawing and can potentially be conducted by the patients themselves. Here, the history of Plasmodium detection is discussed, and advantages and disadvantages of diagnostic methods that are currently being applied are assessed.

show abstract

Innovations in Plasmodium spp. diagnosis on diverse detection platforms

et al. 2021

View full text Add to dashboard Cite

Proof of Concept for a Portable Platform for Molecular Diagnosis of Tropical Diseases

Cited by 23 publications

References 49 publications

Demonstration of a fast and easy sample-to-answer protocol for tuberculosis screening in point-of-care settings: A proof of concept study

Demonstration of a fast and easy sample-to-answer protocol for tuberculosis screening in point-of-care settings: A proof of concept study

Diagnosis of Malaria Parasites Plasmodium spp. in Endemic Areas: Current Strategies for an Ancient Disease

Innovations in Plasmodium spp. diagnosis on diverse detection platforms

Contact Info

Product

Resources

About