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Retrovirus-delivered siRNA

Published by National Institutes of Health | U.S. Department of Health & Human Services | Metadata Last Checked: September 29, 2025 | Last Modified: 2025-09-29
The ability of transfected synthetic small interfering (si) RNAs to suppress the expression of specific transcripts has proved a useful technique to probe gene function in mammalian cells. However, high production costs limit this technology's utility for many laboratories and experimental situations. Recently, several DNA-based plasmid vectors have been developed that direct transcription of small hairpin RNAs, which are processed into functional siRNAs by cellular enzymes. Although these vectors provide certain advantages over chemically synthesized siRNAs, numerous disadvantages remain including merely transient siRNA expression and low and variable transfection efficiency.

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Complete Metadata

bureauCode 
[
  "009:25"
]
identifier https://healthdata.gov/api/views/h9zy-2xip
issued 2025-07-14
landingPage https://healthdata.gov/d/h9zy-2xip
programCode 
[
  "009:033"
]
theme 
[
  "NIH"
]

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