Your search keyword '"Nemudraia A"' showing total 4 results

1. Repair of CRISPR-guided RNA breaks enables site-specific RNA excision in human cells.

Author

Nemudraia, Anna, Nemudryi, Artem, and Wiedenheft, Blake

Subjects

*CRISPRS, *DNA repair, *RNA, *ENDONUCLEASES, *GENOME editing, *DNA

Abstract

Genome editing with CRISPR RNA-guided endonucleases generates DNA breaks that are resolved by cellular DNA repair machinery. However, analogous methods to manipulate RNA remain unavailable. We show that site-specific RNA breaks generated with type-III CRISPR complexes are repaired in human cells and that this repair can be used for programmable deletions in human transcripts to restore gene function. Collectively, this work establishes a technology for precise RNA manipulation with potential therapeutic applications. [ABSTRACT FROM AUTHOR]

Published

2024

2. CRISPR-based engineering of RNA viruses.

Author

Nemudryi, Artem, Nemudraia, Anna, Nichols, Joseph E., Scherffius, Andrew M., Zahl, Trevor, and Wiedenheft, Blake

Abstract

The article discusses the history of DNA manipulation techniques, particularly recombinant DNA, and the development of tools for in vivo editing using site-specific nucleases. It highlights the limitations of current methods for manipulating RNA and introduces a new approach that combines type III CRISPR-based RNA cleavage with splinted RNA ligation to enable precise deletions and insertions in target RNA sequences, with potential applications in RNA virus genome engineering.

Published

2023

3. The Rise and Fall of SARS-CoV-2 Variants and Ongoing Diversification of Omicron.

Author

Wiegand, Tanner, Nemudryi, Artem, Nemudraia, Anna, McVey, Aidan, Little, Agusta, Taylor, David N., Walk, Seth T., and Wiedenheft, Blake

Subjects

*SARS-CoV-2, *SARS-CoV-2 Omicron variant, *VIRAL proteins, *COVID-19, *VIRAL transmission

Abstract

In late December of 2019, high-throughput sequencing technologies enabled rapid identification of SARS-CoV-2 as the etiological agent of COVID-19, and global sequencing efforts are now a critical tool for monitoring the ongoing spread and evolution of this virus. Here, we provide a short retrospective analysis of SARS-CoV-2 variants by analyzing a subset (n = 97,437) of all publicly available SARS-CoV-2 genomes (n = ~11.9 million) that were randomly selected but equally distributed over the course of the pandemic. We plot the appearance of new variants of concern (VOCs) over time and show that the mutation rates in Omicron (BA.1) and Omicron sub-lineages (BA.2–BA.5) are significantly elevated compared to previously identified SARS-CoV-2 variants. Mutations in Omicron are primarily restricted to the spike and nucleocapsid proteins, while 24 other viral proteins—including those involved in SARS-CoV-2 replication—are generally conserved. Collectively, this suggests that the genetic distinction of Omicron primarily arose from selective pressures on the spike, and that the fidelity of replication of this variant has not been altered. [ABSTRACT FROM AUTHOR]

Published

2022

4. CRISPR-Cas, Argonaute proteins and the emerging landscape of amplification-free diagnostics.

Author

Santiago-Frangos, Andrew, Nemudryi, Artem, Nemudraia, Anna, Wiegand, Tanner, Nichols, Joseph E., Krishna, Pushya, Scherffius, Andrew M., Zahl, Trevor R., Wilkinson, Royce A., and Wiedenheft, Blake

Subjects

*ARGONAUTE proteins, *CRISPRS, *COVID-19 pandemic, *FIELD-effect transistors, *MICROFLUIDIC devices, *POLYMERASE chain reaction

Abstract

[Display omitted] • Reliable and rapid direct to consumer diagnostics are necessary to stop the spread of highly contagious infectious agents. • Programable diagnostics that rely on base-pairing are emerging as disruptive new alternatives to PCR. • Nucleic acid-guided proteins are being coupled to reliable and easy to read detection devices. • Standardized reporting metrics will facilitate objective comparisons between platforms. Polymerase Chain Reaction (PCR) is the reigning gold standard for molecular diagnostics. However, the SARS-CoV-2 pandemic reveals an urgent need for new diagnostics that provide users with immediate results without complex procedures or sophisticated equipment. These new demands have stimulated a tsunami of innovations that improve turnaround times without compromising the specificity and sensitivity that has established PCR as the paragon of diagnostics. Here we briefly introduce the origins of PCR and isothermal amplification, before turning to the emergence of CRISPR-Cas and Argonaute proteins, which are being coupled to fluorimeters, spectrometers, microfluidic devices, field-effect transistors, and amperometric biosensors, for a new generation of nucleic acid-based diagnostics. [ABSTRACT FROM AUTHOR]

Published

2022