Difference between revisions of "Part:BBa K4088888"
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'''dCas13a'''<br/> | '''dCas13a'''<br/> | ||
− | LwaCas13a has been reported to mediate more robust RNA-targeting activity than the LshCas13 system but requires a stabilizer fusion, for example, msfGFP for efficient interference activity <ref> Mahas, A., Aman, R. & Mahfouz, M. CRISPR-Cas13d mediates robust RNA virus interference in plants. Genome Biol 20, 263 (2019). doi.org/10.1186/s13059-019-1881-2</ref>. As a stabilizer fusion we use fragments of beta-lactamase thus improving targeting activity. | + | LwaCas13a has been reported to mediate more robust RNA-targeting activity than the LshCas13 system but requires a stabilizer fusion, for example, msfGFP for efficient interference activity <ref> Mahas, A., Aman, R. & Mahfouz, M. CRISPR-Cas13d mediates robust RNA virus interference in plants. Genome Biol 20, 263 (2019). https://doi.org/10.1186/s13059-019-1881-2</ref>. As a stabilizer fusion we use fragments of beta-lactamase thus improving targeting activity. |
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dCas13a is a catalytically dead lwaCas13aenzyme (formerly C2c2) with R407A and R1046A mutations in HEPN-domain. The Cas13 family of enzymes contains at least 4 subtypes, including Cas13a, which is used in this Part. dCas13a interacts with gRNA about 65 nucleotides in length. dCas13a-gRNA complex detects complementary RNA in the sample. dCas13a is very specific variant of RNA detection, it can been customized to recognize single nucleotides on the target RNA. | dCas13a is a catalytically dead lwaCas13aenzyme (formerly C2c2) with R407A and R1046A mutations in HEPN-domain. The Cas13 family of enzymes contains at least 4 subtypes, including Cas13a, which is used in this Part. dCas13a interacts with gRNA about 65 nucleotides in length. dCas13a-gRNA complex detects complementary RNA in the sample. dCas13a is very specific variant of RNA detection, it can been customized to recognize single nucleotides on the target RNA. |
Revision as of 14:04, 21 October 2021
dCas13a-Clact
С-terminal fragment of β-lactamase fused with dCas13a.
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21INCOMPATIBLE WITH RFC[21]Illegal BglII site found at 1580
Illegal BglII site found at 1790
Illegal BglII site found at 2057
Illegal BglII site found at 2822
Illegal XhoI site found at 3751 - 23COMPATIBLE WITH RFC[23]
- 25COMPATIBLE WITH RFC[25]
- 1000COMPATIBLE WITH RFC[1000]
Usage and Biology
β-Lactamase
β-Lactamase (AmpR) - the gene encoding beta-lactamase is a protein known for providing antibiotic resistance of bacteria to ampicillin, because it is able to destroy the beta-lactam ring. This ability allows beta-lactamase to be used as a reporter protein (reaction with nitrocefin, which changes color when the beta-lactam ring is destroyed). Simple, reliable, readily available, it is not difficult to express in cells. These advantages have led us to use this particular reporter protein.
N_lac and C_lac are genes encoding N and C fragments of beta-lactamase, respectively. We selected their sequence in a special way, taking into account the mechanism of protein splicing [1] . For this, we purposefully divided the ampR sequence in front of cysteine (you can also use threonine, the main thing is that they carry nucleophiles in the radical).
Linker
Usually one tries to take neutral amino acids like glycine and alanine as part of the linkers: It is desirable to make the linker neutral. The main thing is without proline, preferably without charged amino acids. Hydrophobic amino acids can be added, e.g. serine. Aliphatic amino acids may also be added. Length: 6-8 amino acids, 10 at most. We use GGGGGG because it meets these criteria. (look at alphafold for it: but it does not start there and gives an error. we even asked our acquaintances to start it with our sequence - without success). So we apparently choose the approach of experimental verification of the linker.
dCas13a
LwaCas13a has been reported to mediate more robust RNA-targeting activity than the LshCas13 system but requires a stabilizer fusion, for example, msfGFP for efficient interference activity [2]. As a stabilizer fusion we use fragments of beta-lactamase thus improving targeting activity.
dCas13a is a catalytically dead lwaCas13aenzyme (formerly C2c2) with R407A and R1046A mutations in HEPN-domain. The Cas13 family of enzymes contains at least 4 subtypes, including Cas13a, which is used in this Part. dCas13a interacts with gRNA about 65 nucleotides in length. dCas13a-gRNA complex detects complementary RNA in the sample. dCas13a is very specific variant of RNA detection, it can been customized to recognize single nucleotides on the target RNA.
References
- ↑ Perler FB. Protein splicing mechanisms and applications. IUBMB Life. 2005 Jul;57(7):469-76. https://doi.org/10.1080/15216540500163343.
- ↑ Mahas, A., Aman, R. & Mahfouz, M. CRISPR-Cas13d mediates robust RNA virus interference in plants. Genome Biol 20, 263 (2019). https://doi.org/10.1186/s13059-019-1881-2