
Ordering Information
| Product Name | Catalog # | UNIT | Price | Qty | FAVORITES | |
MLL3 Lentiviral Activation Particles (h) | sc-402052-LAC | 200 µl | $455.00 | |||
MLL3 Lentiviral Activation Particles (h2) | sc-402052-LAC-2 | 200 µl | $455.00 |
KMT2C (MLL3) encodes a SET domain–containing histone lysine methyltransferase that primarily catalyzes H3K4 monomethylation at enhancers, shaping enhancer–promoter communication and transcriptional output. As a core component of COMPASS-like complexes, MLL3 integrates chromatin cues to regulate lineage specification, differentiation programs, and stimulus-responsive gene expression across multiple signaling contexts. Disruption of KMT2C is frequently observed in cancer genomics and is also implicated in altered epigenetic regulation in developmental and neurobiological disorders, reflecting its role in maintaining transcriptional homeostasis. These properties make MLL3 a key node for studying enhancer regulation, chromatin architecture, and context-dependent transcriptional control in human cells.
MLL3 Lentiviral Activation Particles (h) address this need by packaging the complete synergistic activation mediator (SAM) transcriptional activation system into transduction-ready, high-titer lentiviral particles, enabling efficient KMT2C upregulation across a broader range of human cell types.
MLL3 Lentiviral Activation Particles (h) deliver all functional components of the synergistic activation mediator (SAM) system via lentiviral transduction. The system comprises three particle preparations co-transduced into target cells: one encoding catalytically inactive dCas9 (D10A and N863A mutations) fused to the VP64 transactivation domain with a blasticidin resistance gene; one encoding the MS2-p65-HSF1 fusion protein with a hygromycin resistance gene; and one encoding a target-specific 20 nt sgRNA fused to two MS2 RNA aptamers with a puromycin resistance gene. Following lentiviral transduction and genomic integration of the expression cassettes, the SAM components are stably expressed and assemble at the target locus within the proximal promoter region upstream of the KMT2C transcriptional start site, where VP64, p65, and HSF1 act cooperatively to recruit endogenous transcriptional machinery and drive sustained upregulation of endogenous MLL3 expression. The use of nuclease-inactive dCas9 avoids the introduction of double-strand DNA breaks and preserves the native KMT2C genomic locus and regulatory architecture.
The lentiviral format offers several practical advantages: stable genomic integration supports heritable activation across cell divisions; high-titer particle preparations eliminate the need for in-house viral production; and compatibility with primary, non-dividing, and transfection-resistant cell types expands experimental accessibility. Successful transduction can be confirmed and enriched through triple antibiotic selection using puromycin, hygromycin, and blasticidin.
For Research Use Only. Not Intended for Diagnostic or Therapeutic Use.