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Human TLR4 Reporter HEK293 Cells (NF-κB and IRF)

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HEK-Dual™ hTLR4 Cells

Human TLR4 expressing HEK293 dual reporter cells (NF-κB and IRF pathways)

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3-7 x 10e6 cells

hkd-htlr4
+-
$1,589

NF-κB–SEAP and IRF-Lucia reporter HEK293 cells expressing human TLR4

Signaling pathways in HEK-Dual™ hTLR4 cells
Signaling pathways in HEK-Dual™ hTLR4 cells

HEK-Dual™ hTLR4 cells were engineered from HEK-Dual™ cells, a human embryonic kidney HEK293-derived cell line, to study the Toll-like receptor 4 (TLR4)-dependent NF-κB and IRF responses upon stimulation with lipopolysaccharide (LPS). LPS is a major constituent of the outer membrane of Gram-negative bacteria and the main microbial mediator implicated in the pathogenesis of sepsis and septic shock [1].

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Description

HEK-Dual™ hTLR4 cells feature the stable expression of TLR4, as well as the adapter proteins MD-2 (myeloid differentiation factor 2) and CD14 (cluster of differentiation 14). These cells also express two inducible reporter genes for SEAP (secreted embryonic alkaline phosphatase) and Lucia luciferase. As a result, these cells allow the simultaneous study of the NF-κB pathway, by monitoring the activity of SEAP, and the IRF pathway, by assessing the activity of the secreted Lucia luciferase. Upon TLR4 activation, both reporter proteins are readily measurable in the cell culture supernatant when using QUANTI-Blue™, a SEAP detection reagent, and QUANTI-Luc™ 4 Lucia/Gaussia, a Lucia luciferase detection reagent.

HEK-Dual™ hTLR4 cells are highly responsive to LPS. They show potent NF-κB and IRF responses upon incubation with TLR4-specific ligands, such as smooth LPS-EB Ultrapure (UP) or rough LPS-EK UP, when compared to HEK-Blue™ hTLR4 cells and the control cell line HEK-Dual™ (see figures).

 

Of note, HEK293 cells express endogenous levels of various PRRs, including TLR3 and TLR5, and therefore might respond to their cognate ligands (see figures)

 

Key features

  • Stable expression of human TLR4, MD-2, and CD14
  • Increased and reproducible response to rough and smooth LPS
  • Distinct monitoring of TLR4-dependent NF-κB or IRF activation by assessing the SEAP and Lucia luciferase activities

Applications

  • Detecting sample contamination with LPS
  • Defining the role of TLR4 in LPS-induced signaling pathways 
  • Screening for TLR4 agonists or antagonists

 

1. Godowski, P., 2005. A smooth operator for LPS responses. Nat Immunol 6, 544–546.

Figures

NF-κB responses of HEK-Blue™ hTLR4 vs. HEK-Dual™ hTLR4
NF-κB responses of HEK-Blue™ hTLR4 vs. HEK-Dual™ hTLR4

NF-κB responses of HEK-Blue™ hTLR4 vs. HEK-Dual™ hTLR4​. HEK-Blue™ hTLR4 and HEK-Dual™ hTLR4 cells were stimulated with various TLR4 agonists: LPS-EB Ultrapure (UP) (1 ng/ml), LPS-EK UP (1 ng/ml), LPS-B5 UP (100 pg/ml), or synthetic MPLAs (100 ng/ml). After overnight incubation, the activation of NF-κB was assessed by measuring the activity of SEAP in the supernatant using QUANTI-Blue™ Solution. Data are shown as optical density (OD) at 650 nm (mean ± SEM).

NF-κB responses in hTLR4-expressing HEK-Dual™ -derived cells
NF-κB responses in hTLR4-expressing HEK-Dual™ -derived cells

NF-κB responses in HEK-Dual™ -derived cells. HEK-Dual™ and HEK-Dual™ hTLR4 cells were incubated for 24 hours with cytokines and various TLR agonists: Human TNF-α (NF-κB-positive control, 1 ng/ml), hIFN-β (IRF-positive control, 1000 U/ml), Pam3CSK4 (TLR2 ligand, 100 ng/ml), Poly(I:C) HMW (TLR3 ligand, 1 µg/ml), LPS-EB Ultrapure (UP) (TLR4 ligand, 1 ng/ml), LPS-EK UP (TLR4 ligand, 1 ng/ml), LPS-B5 UP (TLR4 ligand, 100 pg/ml), CRX-527 (TLR4 ligand, 1 ng/ml), MPLAs (TLR4 ligand, 100 ng/ml), FLA-ST UP (TLR5 ligand, 100 ng/ml), R848 (TLR7/8 ligand, 10 µg/ml), or ODN 2006 (TLR9 ligand, 10 µg/ml). After 24h incubation, the NF-kB-induced SEAP activity was assessed using QUANTI-Blue™. Data are shown as optical density (OD) at 650 nm (mean ± SEM).

IRF responses in hTLR4-expressing HEK-Dual™ -derived cells
IRF responses in hTLR4-expressing HEK-Dual™ -derived cells

IRF responses in HEK-Dual™ -derived cells. HEK-Dual™ and HEK-Dual™ hTLR4 cells were incubated for 24 hours with cytokines and various TLR agonists: Human TNF-α (NF-κB-positive control, 10 ng/ml), hIFN-β (IRF-positive control, 10 U/ml), Pam3CSK4 (TLR2 ligand, 100 ng/ml), Poly(I:C) HMW (TLR3 ligand, 100 ng/ml), LPS-EB Ultrapure (UP) (TLR4 ligand, 10 ng/ml), LPS-EK UP (TLR4 ligand, 10 ng/ml), LPS-B5 UP (TLR4 ligand, 1 ng/ml), CRX-527 (TLR4 ligand, 100 ng/ml), MPLAs (TLR4 ligand, 100 ng/ml), FLA-ST UP (TLR5 ligand, 100 ng/ml), R848 (TLR7/8 ligand, 10 µg/ml), or ODN 2006 (TLR9 ligand, 10 µg/ml). After 24h incubation, the IRF response was assessed by measuring the activity of Lucia luciferase in the supernatant using QUANTI-Luc™. Data are shown in fold response over non-induced cells (mean ± SEM).

Inhibition of TLR4-dependent NF-κB and IRF responses using CLI-095
Inhibition of TLR4-dependent NF-κB and IRF responses using CLI-095

Inhibition of hTLR4 signaling pathway using CLI-095. HEK-Dual™ hTLR4 cells were incubated in the presence of increasing concentrations of CLI-095 for 3 hours before adding 10 ng/ml LPS-EK Ultrapure (TLR4 agonist). After overnight incubation, the inhibitory effect of CLI-095 on the NF-κB and IRF pathways was determined by measuring the reduction of SEAP and Lucia production in the supernatant using the QUANTI-Blue™ and QUANTI-Lucia™ detection reagents, respectively. Data are shown as a percentage (%) of maximal TLR4 activation (without inhibitor).

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Specifications

Antibiotic resistance: Blasticidin, Hygromycin, PuromycinZeocin®

Growth medium: DMEM, 4.5 g/l glucose, 2 mM L-glutamine, 10% (v/v) fetal bovine serum, 100 U/ml penicillin, 100 μg/ml streptomycin, 100 μg/ml Normocin™

Quality Control:

  • Stable expression of human TLR4, MD-2, and CD14 has been verified by RT-qPCR and functional assays.
  • The stability for 20 passages, following thawing, has been verified. 
  • These cells are guaranteed mycoplasma-free.

 

These cells are covered by a Limited Use License (See Terms and Conditions).

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Contents

 

dry ice Shipped on dry ice (Europe, USA, Canada and some areas in Asia)

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Details

Toll-like receptor 4 signaling

The Toll-like receptor 4 (TLR4) was the first TLR identified and is an important pattern recognition receptor (PRR) in innate immunity and inflammation. It is found both on the cell surface and in endosomes of innate immune cells including monocytes and macrophages, as well as on intestinal epithelium and endothelial cells [1]. TLR4 can recognize pathogen- and damage-associated molecular patterns (PAMPs and DAMPs). However, it is primarily activated by lipopolysaccharide (LPS) and its toxic moiety Lipid A [2]. TLR4 does not directly interact with LPS, but requires essential adaptor proteins [3]. The soluble LPS-binding protein (LBP) extracts monomeric LPS from the microbial membrane and transfers it to CD14 (cluster of differentiation 14). This membrane-bound protein then interacts with MD-2 (myeloid differentiation factor 2), which is constitutively associated with the TLR4 ectodomain. The ligand-loaded MD-2 subsequently binds to another TLR4/MD-2/LPS complex, leading to their dimerization [4].  Then, TLR4 triggers two distinct signaling cascades [5]:

  • the MyD88-dependent activating NF-κB pathway (at the cell surface) 
  • the TRIF-dependent activating IRF pathway (in endosomes) 

At the cell surface, activation of TLR4 initiates the TIRAP-MyD88-dependent pathway, ultimately leading to the activation of NF-κB and the production of a pro-inflammatory response. Also, the TLR4 complex can be endocytosed into endosomes in a CD14-mediated fashion. This results in the the stimulation of IRF3 (interferon regulatory factor), which modulates the expression of type I IFN [3].

TLR4 signaling is crucial in both acute and chronic inflammatory disorders and thus, is an attractive target for novel treatments [1]. Stimulating drugs are useful for the development of vaccine adjuvants or cancer immunotherapeutics, whereas TLR4-inhibition is a therapeutic approach to treat septic shock or autoimmune inflammatory pathologies such as atherosclerosis [5].

 

LPS structure

 

Rough vs smooth LPS

Lipopolysaccharide (LPS) is a major constituent of the outer membrane of Gram-negative bacteria. It comprises three covalently linked regions:

  • the lipid A (endotoxin)
  • the rough core oligosaccharide
  • the O-antigenic side chain.

 

Wild-type LPS contains the O-side chain and is referred to as smooth (sLPS). Few bacterial strains (e.g. Salmonella Thyphimurium, Brucella canis) lost the O-side chain. This mutated form is called rough (rLPS). Both sLPS and rLPS share the same receptor complex (TLR4-MD-2-CD14), but their mechanism of action differs. While CD14 is necessary for sLPS NF-κB and IRF signaling, it is dispensible for rLPS NF-κB signaling. It has been hypothesized that rLPS activates a broader range of cells (CD14 positive, low and negative), accounting for higher toxicity [6]. 

Nevertheless, both LPS variations elicit potent innate immune responses. The resulting signaling triggers the release of pro‑inflammatory cytokines, which can lead to both acute and chronic inflammatory diseases. It is all about balance: small controlled amounts of LPS can be protective and large uncontrolled amounts can lead to disastrous outcomes, such as septic shock [7]. Despite its highly inflammatory nature, LPS has remarkable therapeutic potential and features many characteristics needed for an effective vaccine adjuvant [8]. 

 

References:

1. Ou, T. et al. 2018. The Pathologic Role of Toll-Like Receptor 4 in Prostate Cancer. Front Immunol 9, 1188.
2. Cochet, F. et al. 2017. The Role of Carbohydrates in the Lipopolysaccharide (LPS)/Toll-Like Receptor 4 (TLR4) Signalling. Int J Mol Sci 18
3. Kuzmich, N.N. et al. 2017. TLR4 Signaling Pathway Modulators as Potential Therapeutics in Inflammation and Sepsis. Vaccines (Basel) 5.
4.Tanimura N. et al. 2014. The attenuated inflammation of MPL is due to the lack of CD14-dependent tight dimerization of the TLR4/MD2 complex at the plasma membrane. Int Immunol.(6):307-14.
5. Romerio A, Peri F. 2020. Increasing the Chemical Variety of Small-Molecule-Based TLR4 Modulators: An Overview. Front Immunol.;11:1210.
6. Zanoni I,.et al., 2012. Similarities and differences of innate immune responses elicited by smooth and rough LPS. Immunol Lett. 2012 Feb 29;142(1-2):41-7.
7. Godowski, P., 2005. A smooth operator for LPS responses. Nat Immunol 6, 544–546.
8. McAleer, J.P. & Vella, A.T., 2010.  Educating CD4 T cells with vaccine adjuvants: lessons from lipopolysaccharide. Trends Immunol 31, 429-435.

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