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RNA therapeutics: function, design, and delivery. Preface.

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Cover of 'RNA therapeutics: function, design, and delivery. Preface.'

Table of Contents

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    Book Overview
  2. Altmetric Badge
    Chapter 1 RNA Modifications: A Mechanism that Modulates Gene Expression
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    Chapter 2 Quantitative Analysis of RNA Modifications
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    Chapter 3 Advances in RNA Sensing by the Immune System: Separation of siRNA Unwanted Effects from RNA Interference
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    Chapter 4 Progress in siRNA delivery using multifunctional nanoparticles.
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    Chapter 5 Optimized Protocols for siRNA Delivery into Monocytes and Dendritic Cells
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    Chapter 6 Systemic delivery of synthetic siRNAs.
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    Chapter 7 What Are the Key Targeted Delivery Technologies of siRNA Now?
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    Chapter 8 Using OligoWalk to Identify Efficient siRNA Sequences
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    Chapter 9 Jet-Injection of Short Hairpin RNA-Encoding Vectors into Tumor Cells
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    Chapter 10 Short Hairpin RNA (shRNA): Design, Delivery, and Assessment of Gene Knockdown
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    Chapter 11 Effective Pol III-Expressed Long Hairpin RNAs Targeted to Multiple Unique Sites of HIV-1
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    Chapter 12 Functional Studies on RNA-Transfected Cell Microarrays
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    Chapter 13 Transfection Microarrays for High-Throughput Phenotypic Screening of Genes Involved in Cell Migration
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    Chapter 14 Intron-Mediated RNA Interference, Intronic MicroRNAs, and Applications
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    Chapter 15 Inhibition of the microRNA Pathway in Zebrafish by siRNA
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    Chapter 16 Profiling of miRNA Expression and Prediction of Target Genes
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    Chapter 17 Small RNA Cloning
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    Chapter 18 In Situ Hybridization Detection of microRNAs
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    Chapter 19 Detection and Quantitative Analysis of Small RNAs by PCR
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    Chapter 20 In Vivo Reprogramming of Human Telomerase Reverse Transcriptase (hTERT) by Trans -Splicing Ribozyme to Target Tumor Cells
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    Chapter 21 Design and Function of Triplex Hairpin Ribozymes
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    Chapter 22 Catalytic M1GS RNA as an antiviral agent in animals.
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    Chapter 23 Using Live Cells to Generate Aptamers for Cancer Study
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    Chapter 24 Primer-Free Aptamer Selection Using a Random DNA Library
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    Chapter 25 Development of TLR7/8 Small RNA Antagonists
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    Chapter 26 Modulation of Dendritic Cell Maturation and Function by siRNA-Bearing 5ʹ-Triphosphate
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    Chapter 27 Immunotherapy of Cancer with Dendritic Cells Loaded with Tumor Antigens and Activated Through mRNA Electroporation
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    Chapter 28 Non-MHC-Dependent Redirected T Cells Against Tumor Cells
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    Chapter 29 Overcoming Self-Tolerance to Tumour Cells
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    Chapter 30 Recent Advances in Hematopoietic Stem Cell Transplantation and Perspectives of RNAi Applications
Attention for Chapter 22: Catalytic M1GS RNA as an antiviral agent in animals.
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Chapter title
Catalytic M1GS RNA as an antiviral agent in animals.
Chapter number 22
Book title
RNA Therapeutics
Published in
Methods in molecular biology, April 2010
DOI 10.1007/978-1-60761-657-3_22
Pubmed ID
Book ISBNs
978-1-60761-656-6, 978-1-60761-657-3
Authors

Bai Y, Rider PJ, Liu F, Yong Bai, Paul Jay Fannin Rider, Fenyong Liu, Bai, Yong, Rider, Paul Jay Fannin, Liu, Fenyong

Abstract

The use of RNase P ribozyme (M1GS catalytic RNA) for inhibition of murine cytomegalovirus (MCMV) propagation in mice is described in this chapter. General information about RNase P based technology is included and followed by detailed protocols focused on (1) construction and in vitro cleavage assay of the customized M1GS ribozyme, (2) stable expression of the M1GS RNA and evaluation of its activity in inhibition of viral gene expression and growth in cultured cells, and (3) investigation of M1GS-mediated inhibition of viral infection and pathogenesis in animals. Using these methods, we have successfully constructed catalytic M1-1 RNA against the MCMV assembly protein (mAP) and M80 mRNA. Our recent study has demonstrated that an 80% reduction in the expression of mAP and M80 and a 2,000-fold reduction in viral growth were observed in cells expressing the ribozyme. Furthermore, after the functional ribozyme-expressing constructs were delivered into MCMV-infected SCID mice, a significant reduction of viral gene expression and infection was detected, and the survival of the infected animals was significantly improved. Collectively, our data demonstrate the feasibility of the use of RNase P ribozyme for inhibition of viral gene expression in animals and support the utility of RNase P ribozyme for gene-targeting applications in vivo.

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Mendeley readers

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Geographical breakdown

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Readers by professional status Count As %
Student > Ph. D. Student 1 50%
Unknown 1 50%
Readers by discipline Count As %
Agricultural and Biological Sciences 1 50%
Unknown 1 50%
Attention Score in Context

Attention Score in Context

This research output has an Altmetric Attention Score of 1. This is our high-level measure of the quality and quantity of online attention that it has received. This Attention Score, as well as the ranking and number of research outputs shown below, was calculated when the research output was last mentioned on 26 January 2012.
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#15,241,801
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Outputs from Methods in molecular biology
#5,280
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Outputs of similar age
#77,141
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Outputs of similar age from Methods in molecular biology
#5
of 14 outputs
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