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Cre In Vitro Transcribed mRNA-LNP
Cre In Vitro Transcribed mRNA-LNP
MRNA-TG-026
Cre In Vitro Transcribed mRNA-LNP
Source:In vitro transcribed mRNA encapsulated with LNP
SKU:MRNA-TG-026-DCPS
Product Name:Cap1-Cre-120nt PolyA Tail In Vitro Transcribed mRNA
Product Description:In Vitro Transcribed mRNA encoding CreORF with Cap1 and 120nt PolyA tail.
SKU:MRNA-TG-026-DCPS
Product Name:Cap1-Cre-120nt PolyA Tail In Vitro Transcribed mRNA
Product Description:In Vitro Transcribed mRNA encoding CreORF with Cap1 and 120nt PolyA tail.
PROPERTIES
Cap:
Cap 1
5'-UTR:
5' -untranslated region derived from human alpha-globin RNA with an optimized Kozak sequence
ORF:
Cre
3'-UTR:
3' UTR comprising two sequence elements derived from the aminoterminal enhancer of split (AES) mRNA and the mitochondrial encoded 12S ribosomal RNA
Poly(A) Tail:
A 110-nucleotide poly(A)-tail consisting of a stretch of 30 adenosine residues, followed by a 10-nucleotide linker sequence and another 70 adenosine residues.
Modifications:
N1-methyl-pseudouridine
Neutral Lipid:
1,2-distearoyl-sn-glycero-3-phosphocholine (DSPC)
Cholesterol:
Cholesterol
Lonizable Lipid:
1,2-dimyristoyl-rac-glycero-3-methoxypolyethylene glycol-2000 (PEG2000-DMG)
PEG-lipid:
Heptadecan-9-yl 8-((2-hydroxyethyl)(8-(nonyloxy)− 8-oxooctyl)amino)octanoate)(SM-102)
Storage:
-20 °C
Buffer:
PBS, pH7.4
Cryoprotectant:
Trehalose
Related Categories
Reporter Gene mRNA
Background

Background

Cre Recombinase is a Type I topoisomerase from bacteriophage P1 that catalyzes the site-specific recombination of DNA between loxP sites. The enzyme requires no energy cofactors and Cre-mediated recombination quickly reaches equilibrium between substrate and reaction products. The loxP recognition element is a 34 base pair (bp) sequence comprised of two 13 bp inverted repeats flanking an 8 bp spacer region which confers directionality. Recombination products depend on the location and relative orientation of the loxP sites. Two DNA species containing single loxP sites will be fused. DNA between directly repeated loxP sites will be excised in circular form while DNA between opposing loxP sites will be inverted with respect to external sequences.

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