Optimisation of an asymmetric polymerase chain reaction assay for the amplification of single-stranded DNA from Wuchereria bancrofti for electrochemical detection

Vasuki, V.; Hoti, S.L.; Kamaraj, Nagalakshmi; Ghosh, Somnath; Rajaram, Kaushik

doi:10.1590/0074-0276108062013020

Cited by 7 publications

(6 citation statements)

References 14 publications

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“…This study aimed to investigate the optimum conditions to achieve the highest yield of highly pure ssDNA using asymmetric PCR. Carrying out of various studies to optimize asymmetric PCR suggests that this process is somewhat difficult, and also it is not possible to consider a single protocol for all random DNA libraries . The first step to get success in asymmetric PCR is the quality of designed library.…”

Section: Discussionmentioning

confidence: 99%

“…It is referred to the high purity of ssDNA template used at the first round. It seems that dsDNA remaining in the templates of round 2 and others can play a role similar to reverse primer and prepare the conditions for maximum activity of forward primer . While the primary library used in the first round is single stranded and lacks any complementary sequence, so reverse primers should make the template for PCR procedure at early cycles.…”

Section: Discussionmentioning

confidence: 99%

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Essential strategies to optimize asymmetric PCR conditions as a reliable method to generate large amount of ssDNA aptamers

Heiat

Ranjbar

Latifi

et al. 2017

Biotech and App Biochem

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Asymmetric PCR, a simple method to generate single-stranded DNA (ssDNA) aptamers in systematic evaluation of ligand by exponential enrichments rounds, is coupled with limitations. We investigated the essential strategies for optimization of conditions to perform a high-quality asymmetric PCR. Final concentrations of primers and template, the number of PCR cycles, and annealing temperature were selected as optimizing variables. The qualities of visualized PCR products were analyzed by ImageJ software. The highest proportion of interested DNA than unwanted products was considered as optimum conditions. Results revealed that the best values for primers ratio, final template concentration, annealing temperature, and PCR cycles were, respectively, 30:1, 1 ng/μL, 55 °C, and 20 cycles for the first and 50:1, 2 ng/μL, 59 °C, and 20 cycles for other rounds. No significant difference was found between optimized asymmetric PCR results in the rounds of two to eight (P > 0.05). The ssDNA quality in round 10 was significantly better than other rounds (P < 0.05). Generally, the ssDNA product with less dimers, double-stranded DNA (dsDNA), and smear are preferable. The dsDNA contamination is the worst, because it can act as antidote and inhibits aptameric performance. Therefore, to choose the best conditions, the lower amount of dsDNA is more important than other unwanted products.

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Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Essential strategies to optimize asymmetric PCR conditions as a reliable method to generate large amount of ssDNA aptamers

Heiat

Ranjbar

Latifi

et al. 2017

Biotech and App Biochem

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show abstract

“…aPCR is one of the most extensively used methods for the direct production of short ssDNA aptamers [ 90 , 93 , 94 , 95 , 96 ]. Due to its highly specific reaction conditions and several limitations, this method was originally limited to the production of ssDNA with ten to a few hundred bases [ 94 , 97 ].…”

Section: Current Methods For Ssdna Scaffold Productionmentioning

confidence: 99%

Synthesis of DNA Origami Scaffolds: Current and Emerging Strategies

et al. 2020

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DNA origami nanocarriers have emerged as a promising tool for many biomedical applications, such as biosensing, targeted drug delivery, and cancer immunotherapy. These highly programmable nanoarchitectures are assembled into any shape or size with nanoscale precision by folding a single-stranded DNA scaffold with short complementary oligonucleotides. The standard scaffold strand used to fold DNA origami nanocarriers is usually the M13mp18 bacteriophage’s circular single-stranded DNA genome with limited design flexibility in terms of the sequence and size of the final objects. However, with the recent progress in automated DNA origami design—allowing for increasing structural complexity—and the growing number of applications, the need for scalable methods to produce custom scaffolds has become crucial to overcome the limitations of traditional methods for scaffold production. Improved scaffold synthesis strategies will help to broaden the use of DNA origami for more biomedical applications. To this end, several techniques have been developed in recent years for the scalable synthesis of single stranded DNA scaffolds with custom lengths and sequences. This review focuses on these methods and the progress that has been made to address the challenges confronting custom scaffold production for large-scale DNA origami assembly.

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“…67,68 Modied RT-PCR amplication, known as asymmetric PCR, coupled with a DNA sensor has been extensively used due to its higher sensitivity, as it generates an excess amount of the ssDNA target for direct hybridization with an immobilized-DNA-probe-modied electrode. [69][70][71][72][73][74] The reverse-to-forward (R/F) concentration ratio is an important part of the asymmetric PCR protocol for creating excess ssDNA production. 75 This is because in asymmetric PCR, the primer with a lower concentration is involved in the production of dsDNA, whereas the primer with a higher concentration (which does not bind to any template) is responsible for the production of ssDNA.…”

Section: The Effects Of Sonication Time On Amplied Genomic Dengue Virus Gene Samplesmentioning

confidence: 99%

Strategies for the preparation of non-amplified and amplified genomic dengue gene samples for electrochemical DNA biosensing applications

et al. 2022

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Optimisation of an asymmetric polymerase chain reaction assay for the amplification of single-stranded DNA from Wuchereria bancrofti for electrochemical detection

Cited by 7 publications

References 14 publications

Essential strategies to optimize asymmetric PCR conditions as a reliable method to generate large amount of ssDNA aptamers

Essential strategies to optimize asymmetric PCR conditions as a reliable method to generate large amount of ssDNA aptamers

Synthesis of DNA Origami Scaffolds: Current and Emerging Strategies

Strategies for the preparation of non-amplified and amplified genomic dengue gene samples for electrochemical DNA biosensing applications

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