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British Journal of Pharmacology logoLink to British Journal of Pharmacology
. 2019 Jun 17;176(15):2736–2749. doi: 10.1111/bph.14695

Inhibitors of DAG metabolism suppress CCR2 signalling in human monocytes

Priscilla Day 1, Lisa Burrows 1, David Richards 1, Samuel J Fountain 1,
PMCID: PMC6609539  PMID: 31032885

Abstract

Background and Purpose

CCL2 is an inflammatory chemokine that stimulates the recruitment of monocytes into tissue via activation of the GPCR CCR2.

Experimental Approach

Freshly isolated human monocytes and THP‐1 cells were used. Fura‐2 loaded cells were used to measure intracellular Ca2+ responses. Transwell migration to measure chemotaxis. siRNA‐mediated gene knock‐down was used to support pharmacological approaches.

Key Results

CCL2 evoked intracellular Ca2+ signals and stimulated migration in THP‐1 monocytic cells and human CD14+ monocytes in a CCR2‐dependent fashion. Attenuation of DAG catabolism in monocytes by inhibiting DAG kinase (R59949) or DAG lipase (RHC80267) activity suppressed CCL2‐evoked Ca2+ signalling and transwell migration in monocytes. These effects were not due to a reduction in the number of cell surface CCR2. The effect of inhibiting DAG kinase or DAG lipase could be mimicked by addition of the DAG analogue 1‐oleoyl‐2‐acetyl‐sn‐glycerol (OAG) but was not rescued by application of exogenous phosphatidylinositol 4,5‐bisphosphate. Suppressive effects of R59949, RHC80267, and OAG were partially or fully reversed by Gö6983 (pan PKC isoenzyme inhibitor) but not by Gö6976 (PKCα and PKCβ inhibitor). RNAi‐mediated knock‐down of DAG kinase α isoenzyme modulated CCL2‐evoked Ca2+ responses in THP‐1 cells.

Conclusions and Implications

Taken together, these data suggest that DAG production resulting from CCR2 activation is metabolised by both DAG kinase and DAG lipase pathways in monocytes and that pharmacological inhibition of DAG catabolism or application suppresses signalling on the CCL2–CCR2 axis via a mechanism dependent upon a PKC isoenzyme that is sensitive to Gö6983 but not Gö6976.

Abbreviations

CCL2

monocyte chemoattractant protein 1/chemokine ligand 2

PBMCs

peripheral blood mononuclear cells

What is already known

  • CCL2‐mediated monocyte recruitment to tissue is involved in the onset and development of several chronic inflammatory diseases.

What this study adds

  • Pharmacological inhibition of DAG metabolism is a novel route to attenuate CCL2 signalling in human monocytes.

What is the clinical significance

  • Possible therapeutic route in inflammatory diseases with sustained monocyte tissue recruitment.

1. INTRODUCTION

Chemokines are low MW extracellular signalling peptides secreted by tissue either constitutively during homeostasis or de novo during an inflammatory response (Griffith, Sokol, & Luster, 2014). They are a diverse family of peptides (CC, CXC, CX3C, and XC chemokines) with a key role in the tissue recruitment and interstitial migration of leukocytes and other cell types, as well as acting both as chemoattractants and as cues for cellular arrest (Alon & Feigelson, 2012; Serbina & Pamer, 2006). The biological affects of chemokines are exerted through the activation of GPCRs expressed on the cell surface of target cells. In addition to beneficial roles in homeostasis and immunity (Luther et al., 2002), the activity of chemokines is also associated with the onset and progression of chronic inflammatory diseases including atherosclerosis and rheumatoid arthritis (Zernecke & Weber, 2010). To this end, several drug discovery programmes have been initiated in an effort to pharmacologically intervene in chemokine receptor signalling for therapeutic benefit. Targeting single chemokine receptors has proven to be difficult to translating to clinical efficiency, likely due to a level of redundancy between chemokine receptor subtypes. Dual therapy has been proposed as a strategy to overcome this, in addition to targeting convergent second messenger pathways (Horuk, 2009).

The chemokine CCL2 (monocyte chemoattractant protein‐1; MCP‐1) activates CCR2, a Gi‐coupled GPCR that elevates intracellular Ca2+ responses and inhibits adenylate cyclase activity (Campwala, Sexton, Crossman, & Fountain, 2014). Classical CD14+/CD16 blood monocytes express high levels of cell surface CCR2 (Weber et al., 2000), in comparison to nonclassical CD14+/CD16+ monocytes. In animal models of atherosclerosis, it has been demonstrated that CCL2 signalling via CCR2 plays an important role in the size of monocyte/macrophage vascular wall infiltrate and size of atherosclerotic lesion (Boring, Gosling, Cleary, & Charo, 1998; Gu et al., 1998; Lutgens et al., 2005; Veillard et al., 2005). CCL2 is also presented on the cell surface of vascular endothelium and participates in monocyte recruitment by stimulating firm adhesion and transmigration to the subendothelial space (Ashida, Arai, Yamasaki, & Kita, 2001; Maus et al., 2002; Wang et al., 1995). The importance of CCL2–CCR2 signalling does not match by our understanding of the signal transduction mechanisms that regulate functional responses in human monocytes (Cronshaw, Owen, Brown, & Ward, 2004; Webb et al., 2008).

Chemokines including CCL2 elicit intracellular Ca2+ responses in leukocytes and other cell types (Campwala et al., 2014; Korniejewska, McKnight, Johnson, Watson, & Ward, 2011). The responses are pertussis toxin‐sensitive and dependent upon PLC (Campwala et al., 2014). The involvement of PLC suggests that DAG would be generated during generation of CCL2‐evoked Ca2+ responses. DAG is a second messenger in its own right and can modulate the activity of PKC and several ion channels. Once produced by cells, DAG is rapidly metabolised by two major pathways: (a) conversion to phosphatidic acid by DAG kinase and (b) hydrolysis to free fatty acid and monoacylglycerol by DAG lipase (Reisenberg, Singh, Williams, & Doherty, 2012). The aim of this study was to investigate the role of DAG metabolising enzymes on CCL2‐evoked intracellular Ca2+ responses and cellular function in human monocytes.

2. METHODS

2.1. Isolation of CD14+ monocyte from human peripheral blood

All work was undertaken with the approval of the Faculty of Medicine and Health Sciences Research Ethics Committee, University of East Anglia, and NHS Health Research Authority Ethics Committee. Healthy volunteer donor blood (National Health Service Blood and Transplant; Addenbrooke's Hospital, Cambridge University Hospital, UK) was used for the preparation of peripheral blood mononuclear cells (PBMCs) using methodology previously described (Layhadi, Turner, Crossman, & Fountain, 2018). In brief, blood was layered on top of Histopaque‐1077 (Sigma Aldrich, Haverhill, UK) for centrifugation at 1,000× g for 25 min. Buffy coat layers were collected, and PBMCs were counted. CD14+ monocytes were positively selected from PBMC using anti‐CD14+ magnetic beads (Miltenyi Biotech). Monocytes were resuspended in salt buffered solution (SBS) buffer (mM): NaCl, 130; KCl, 5; MgCl2, 1.2; CaCl2, 1.5; d‐glucose, 8; HEPES, 10; pH 7.4.

2.2. Culture of THP‐1 human monocyte cells

THP‐1 monocyte cells (CLS Cat# 300356/p804_THP‐1, RRID:CVCL_0006) were cultured at 37°C, 5% CO2 in RPMI 1640 medium containing 2‐mM l‐glutamine and supplemented with 10% (v/v) FBS, 50‐IU·ml−1 penicillin, and 50‐μg·ml−1 streptomycin. Cells densities were maintained between 1 × 105 and 1 × 106 cells·ml−1.

2.3. Intracellular Ca2+ measurements

Experiments were conducted as described previously (Micklewright, Layhadi, & Fountain, 2018). Briefly, cells were treated with antagonists or vehicle controls for 30 min prior to challenge with agonists. Measurements were made using a 96‐well plate reader with rapid well injection (Flexstation III, Molecular Devices). All experiments were performed in SBS (pH 7.4), containing 130‐mM sodium chloride, 5‐mM potassium chloride, 1.2‐mM magnesium chloride, 1.5‐mM calcium chloride, 8‐mM d‐(+)‐glucose, and 10‐mM HEPES. The cells were then loaded with 2‐μM Fura‐2AM (TEF Labs, Austin, TX, USA) in SBS supplemented with 0.01% (w/v) pluronic for 1 hr at 37°C while being protected from light. The loading buffer was then removed, and the cells were washed twice with SBS. Where applicable, the cells were incubated for a further 30 min with antagonists/vehicle or calcium‐free SBS (SBS lacking 1.5‐mM calcium chloride but containing 2‐mM EGTA, pH 7.4). All antagonists were dissolved in water or DMSO. Changes in intracellular Ca2+ concentration were measured as the ratio of emission at 510 nm following excitation at 340 and 380 nm (F ratio). Cells were treated with antagonists or vehicle controls for 30 min prior to challenge with agonists.

2.4. Flow cytometry

All sets were conducted at room temperature; 1 × 106 cells·ml−1 were prepared in 100‐μl PBS for each marker and control experiment. Cells were treated for 30 min with drugs and vehicle controls prior to being labeled with an antibody. Cells were incubated with 5‐μg·ml−1 human BD Fc block (BD Pharmingen, New Jersey, USA) for 10 min. Next, (1:100) mouse monoclonal anti‐CCR2 PE‐conjugated antibody (BioLegend Cat# 357205, RRID:AB_2562058) or isotype control (BioLegend, USA) was added, and cells were incubated in the dark for 30 min. Labelled cells were analysed using a CytoFLEX flow cytometer (Beckman Coulter). Fluorescence intensity was read for PE using 496‐nm excitation and 578‐nm emission wavelengths, respectively. Living cells were gated according to their forward and side scatter profiles, and then histograms were plotted to compare fluorescence intensity for anti‐CCR2 and isotype control antibodies using CytExpert Software (version 1.2.11, Beckman Coulter).

2.5. siRNA‐mediated gene knock‐down

THP‐1 cells (2 × 105 final) were incubated overnight in complete RPMI (10% FBS) without antibiotics before cells were transfected using Dharmacon siRNA (25‐nM final concentration) with DharmaFECT 2 transfection reagent (Dharmacon Research Inc, Cambridge, UK) using the manufacturer's protocol for a 96‐well format. Scrambled siRNA and siRNA targeted against GAPDH were used in negative and positive control experiments, respectively.

2.6. RNA extraction and nonquantitative RT‐PCR

Total RNA was extracted from cells using Tri Reagent (Sigma Aldrich) with subsequent DNase I treatment (Ambion). cDNA was synthesised from 1‐μg total RNA using Superscript II reverse transcriptase (Invitrogen, Waltham, USA). PCR was performed using a Taq polymerase readymix (Sigma Aldrich) using the primers as given in Table 1.

Table 1.

Expression of DAG kinase, DAG lipase, and PKC mRNA transcripts in CD14+ monocytes and THP‐1 cells

Gene Name CD14+ monocytes THP‐1 cells
DGKA DAG kinase α Expressed Expressed
Sense CAACAGGAGGCAAAACTGGC
Anti‐sense TGCCACCTAGAGATCCACGA
DGKB DAG kinase β Not expressed Not expressed
Sense TCTGTGTGCAATGGAGGCAT
Anti‐sense CCACCCACAACAATCTGTCCA
DGKD DAG kinase δ Expressed Expressed
Sense TTATTGGTTGCACGCACAGC
Anti‐sense CAGACCATCATCAAAGAGGGGA
DGKE DAG kinase ε Expressed Expressed
Sense AGAGGGTAAGTCTCGTCCCC
Anti‐sense CTCTGGGAACAGGCAACGAT
DGKG DAG kinase γ Expressed Expressed
Sense GACTTCTCACCTGGCCTGTC
Anti‐sense GTCCCTCGGTCTTCAAGCTC
DGKH DAG kinase η Expressed Expressed
Sense TATCCCCAGATCCAGGCTGT
Anti‐sense CAGATGCAGCTATGCTCCCA
DGKI DAG kinase ι Not expressed Not expressed
Sense TCCAGTGTGACATGGGCATC
Anti‐sense GGTACCTGAATCCACGGCAA
DGKK DAG kinase κ Expressed Not expressed
Sense CACTGGGCAATGCGATGATG
Anti‐sense TAACCAGACAAGCCCACGAC
DGKQ DAG kinase θ Expressed Expressed
Sense AGGCTCCGAGAGTGACTGAT
Anti‐sense GTGAACCCCAAGAGTGGAGG
DGKZ DAG kinase ζ Expressed Expressed
Sense GGCTCAGGTCGAAGACTTGT
Anti‐sense CAGGATGCTGCAGAAGTCAGT
DAGLA DAG lipase α Expressed Expressed
Sense TGTCGGATGGCACAATGTCA
Anti‐sense GAGCCCAGGATGGAGGTGG
DAGLB DAG lipase β Expressed Expressed
Sense GTTCGTACCACAAACCGTGC
Anti‐sense CTCCCAGGAAGCTGATCTGGA
PRKCA PKCα Expressed Expressed
Sense CCTTTGCCACACACTTTGGG
Anti‐sense TGACCGAGTGAAACTCACGG
PRKCB PKCβ Expressed Expressed
Sense TCTCTTGTCTCTAGCTTTTGGCT
Anti‐sense CCCGGAAGAAAAGACGACCA
PRKCG PKCγ Not expressed Not expressed
Sense TCTAGAATGGGACAGGGGGT
Anti‐sense CAGGACAGCCTCCCTTCGAT
PRKCD PKCδ Expressed Expressed
Sense TGTTGAGGCCCCAGACAAAG
Anti‐sense TGGTGGTTGGTGCGTTGTAG
PRKCE PKCε Expressed Expressed
Sense GGTGCAGACTTGACACTGGT
Anti‐sense GAACCCGGCGAGGAAATACA
PRKCH PKCη Not expressed Expressed
Sense GATCCACCCAACCCTCGAA
Anti‐sense GCGGGGGTTCTGTGAACTTG
PRKCQ PKCθ Expressed Expressed
Sense TTAAGCAGCGAGCCTGTTGA
Anti‐sense GAAACCTCAAGGCCGAATGC
PRKCI PKCι Expressed Expressed
Sense CCCTGGTGTTCATTGCCTCT
Anti‐sense GGCCTTTGCAATGAGGTTCG
PRKCZ PKCζ Expressed Expressed
Sense TGGCTTAAGGTCCTCCGAGT
Anti‐sense GAGTTCCGCGGAGTTGACC
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Note. Data are representative of five donors/independent experiments. Sense and anti‐sense primer sequences used for nonquantitative RT‐PCR are given beneath each gene assayed. Positive control PCR products were generated for all primers sets using human brain cDNA template.

2.7. Immunocytochemistry

THP‐1 cells were seeded onto poly l‐lysine coated coverslips followed by fixation with 4% (w/v) paraformaldehyde for 15 min at room temperature and permeabilisation with 0.25% (v/v) Triton X‐100 for 10 min. Fixed and permeabilised cells were blocked with 1% (w/v) BSA. Cells were incubated with primary antibodies overnight at 4°C, followed by washing and incubation with Alexa Fluor 488‐conjugated secondary antibodies. In negative control experiments, primary antibodies were omitted. Rabbit polyclonal primary antibodies (anti‐DGKδ, Sigma HPA049101, RRID:AB_2680630; anti‐DGKγ, Abcam ab151967, RRID:AB_151967; anti‐DGKη, Abcam ab80693, RRID:AB_1658681; anti‐DGKζ, Abcam ab111047, RRID:AB_10858121; anti‐DAGLα, Abcam ab106979, RRID:AB_10862875; and anti‐DAGLβ) were used in conjunction with a goat anti‐rabbit secondary antibody (Thermo Fisher Scientific Cat# A27034, RRID:AB_2536097). Mouse monoclonal primary antibodies (anti‐PKCα, Santa Cruz Biotechnology sc‐8393, RRID:AB_628142; anti‐DGKα, Santa Cruz Biotechnology sc‐271644, RRID:AB_10708574; anti‐DGKε, Santa Cruz Biotechnology Cat# sc‐100372, RRID:AB_2245858; and anti‐DGKθ, Santa Cruz Biotechnology sc‐137197, RRID:AB_2292802) were used in conjunction with goat anti‐mouse secondary antibody (Thermo Fisher Scientific Cat# A28175, RRID:AB_2536161). Fluorescent and brightfield images were captured using a Zeiss AxioPlan 2ie epifluorescent microscope. The Immuno‐related procedures used comply with the recommendations made by the British Journal of Pharmacology.

2.8. Transmigration assays

Transwell migration assays were performed as previously described (Micklewright et al., 2018). Briefly, assays were performed in 24‐well plates using polyethylene terephthalate membrane inserts with 3‐μm pores; 1 × 106 cells in RPMI (no serum), with vehicle or drug treatment added to the lower chamber. Assays were performed for 2 hr at 37°C, and the cells that had migrated were on the underside of the transwell insert membrane and were stained using crystal violet. The chemotactic index was calculated as the ratio of cells that migrated towards CCL2 over vehicle control. These experiments were blinded.

2.9. DAG assay

DAG levels were measured using an enzyme‐linked fluorescence assay (Cell Biolabs). Accumulation of fluorescence product was measured using 530‐nm excitation and 590‐nm emission; 5 × 107 THP‐1 cells in suspension were incubated at 20°C in SBS solution for 2 hr prior to CCL2 challenge. Cells were exposed to inhibitors for 30 min before challenge with CCL2 or vehicle. Following cell exposure to CCL2 for 1 or 2 min, cells were plunged on ice and sonicated in methanol, followed by extraction of organic phase in chloroform. Total protein was measured by the Bradford assay and used to normalise fluorescence measurements.

2.10. Cell toxicity assay

Potential cytotoxic effects of drug treatments were measured by quantification of LDH release from cells using a colorimetric assay (Abcam) as described by Campwala et al. (2014). To mimic experimental conditions, 1 × 106 THP‐1 or freshly isolated monocytes were incubated with test compounds in SBS assay buffer for 30 min prior to conducting the LDH assay; 0.1% Triton X‐100 was used in positive control experiments. These experiments were blinded.

2.11. Data and statistical analysis

The data and statistical analysis comply with the recommendations on experimental design and analysis in pharmacology (Curtis et al., 2018). Data analysis was performed using Origin Pro 9.0 software (Origin Lab, USA). Dose–response curves were fitted assuming an n H of 1, with the Hill equation used to determine the degree of cooperation. Figure data points represent mean values ± SEM (error bars); n is defined as number of technical repeats or biological repeats (donor number) for experiments with THP‐1 cells and freshly isolated CD14+ monocytes, respectively. Statistical significance was determined using Student's paired t test for two samples and ANOVA for multiple sample datasets. A confidence interval of 5% (P < .05) is applied throughout.

2.12. Blinding in experiments

Experimental manipulations were blinded to the experimenter where technically feasible.

2.13. Chemicals and reagents

Unless otherwise stated, all chemicals and reagents were purchased from Sigma Aldrich.

2.14. Nomenclature of targets and ligands

Key protein targets in this article are hyperlinked to corresponding entries in http://www.guidetopharmacology.org, the common portal for data from IUPHAR/BPS Guide to PHARMACOLOGY (Harding et al., 2018), and are permanently archived in the Concise Guide to PHARMACOLOGY 2017/2018 (Alexander, Christopoulos et al., 2017; Alexander, Fabbro et al., 2017).

3. RESULTS

3.1. DAG kinase and DAG lipase inhibitors attenuate CCL2‐evoked intracellular Ca2+ signals and migration in freshly isolated human monocytes and THP‐1 monocytic cells

CCL2 evoked concentration‐dependent intracellular Ca2+ responses in freshly isolated human CD14+ monocytes (Figure 1a) with an EC50 of 33 ± 4 nM (n = 8; Figure 1b). These responses were abolished by the CCR2 selective antagonist BMSCCR222 (Figure 1c; IC50 9.2 ± 1.2 nM, n = 8). CCL2 also evoked Ca2+ responses in THP‐1 monocytes (Figure 1d) with an EC50 45 ± 12 nM (n = 6; Figure 1e), and these responses were abolished by BMSCCR222 (Figure 1f; IC50 8.4 ± 1.4 nM, n = 6). These data demonstrate that CCL2‐evoked intracellular Ca2+ responses are dependent upon CCR2 activation in both freshly isolated monocytes and the THP‐1 monocytic cells. CCL2‐evoked intracellular Ca2+ responses in freshly isolated monocytes (Figure 1a) and THP‐1 monocytic cells (Figure 1d) were abolished following PLC inhibition with U73122.

Figure 1.

Figure 1

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CCR2 is the cognate receptor for CCL2 in freshly isolated human monocytes and THP‐1 monocytic cells. (a) Averaged (n = 8) intracellular Ca2+ response to CCL2 (50 ng·ml−1) in freshly isolated CD14+ human monocytes. Response in the presence (open circles) and absence (closed circles) of 5‐μM U73122 (n = 6; P < .05). (b) Concentration–response curve for CCL2‐evoked responses in freshly isolated monocytes (n = 8; EC50 = 33 ± 4 nM). (c) Concentration–inhibition curve for selective CCR2 antagonist BMSCCR222 (IC50 = 9 ± 1 nM; n = 8) against Ca2+ responses evoked by CCL2 (50 ng·ml−1) in freshly isolated monocytes. (d) Averaged (n = 6) intracellular Ca2+ response to CCL2 (50 ng·ml−1) in THP‐1 cells. Response in the presence (open circles) and absence (closed circles) of 5‐μM U73122 (n = 6; P < .05). (e) Concentration–response curve for CCL2‐evoked responses in THP‐1 cells (n = 6; EC50 = 45 ± 12 nM). (f) Concentration–inhibition curve for BMSCCR222 (IC50 = 8 ± 1 nM; n = 6) against Ca2+ responses evoked by CCL2 (50 ng·ml−1) in THP‐1 cells. F ratio is the Ca2+ response as measured by the Fura‐2 emission intensity ratio when excited at 340 and 380 nm. Data in concentration–response/inhibition curves are expressed as a percentage of the control response in the presence of vehicle alone

CCR2 is a Gi‐coupled GPCR that elicits intracellular Ca2+ responses in a pertussis toxin‐sensitive and PLC‐dependent fashion (Campwala et al., 2014). This signal transduction mechanism generates DAG, and we therefore investigated the impact of DAG metabolism on CCL2‐evoked Ca2+ responses. In THP‐1 monocytes, R59949 (a small molecule inhibitor of DAG kinase; de Chaffoy de Courcelles et al., 1989) attenuated CCL2‐evoked Ca2+ signalling (Figure 2a) with a half‐maximal concentration of 8.6 ± 1.2 μM (n = 7; Figure 2b). Maximal response in THP‐1 cells was inhibited by approximately 70% using 30‐μM R59949 (Figure 2c). Similarly, CCL2‐evoked Ca2+ responses were suppressed by RHC80267 (Figure 2d), an inhibitor of DAG lipase (Dale & Penfield, 1987). RHC80267 inhibited the response with a half‐maximal concentration of 9.3 ± 1.0 μM (n = 7; Figure 2e), reducing the maximal response to CCL2 by approximately 30% using 30‐μM RHC80267 (Figure 2f). In addition to CCL2‐evoked Ca2+ signals, inhibition of both DAG kinase and DAG lipase attenuated CCL2‐mediated THP‐1 chemotaxis (Figure 2g). Application of CCL2 to THP‐1 monocytic cells caused a rapid increase in cellular DAG (Figure 2h). As for CCL2‐evoked Ca2+ signals (Figure 1d), PLC inhibition with U73122 attenuated the CCL‐2 evoked increase in cellular DAG (Figure 2h). Both R59949 and RHC80267 significantly enhanced CCL2‐evoked DAG elevation (Figure 2h), consistent with a role of DAG kinase and DAG lipase in metabolising DAG following receptor‐mediated synthesis.

Figure 2.

Figure 2

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Inhibitors of DAG kinase and DAG lipase attenuate CCL2‐evoked Ca2+ signalling and migration in THP‐1 cells. (a) Effect of DAG kinase inhibitor R59949 (30 μM) on Ca2+ responses evoked by CCL2 (50 ng·ml−1; n = 7). Averaged responses are shown in the presence of vehicle (closed circles) and inhibitor (open circles). (b) R59949 concentration–inhibition curve (IC50 = 9 ± 1 μM; n = 7) against Ca2+ responses evoked by CCL2 (50 ng·ml−1). (c) Effect of 30‐μM R59949 on CCL2 concentration–response curve (n = 7). (d) Effect of DAG lipase inhibitor RHC80267 (30 μM) on Ca2+ responses evoked by CCL2 (50 ng·ml−1; n = 7). Averaged responses are shown in the presence of vehicle (closed circles) and inhibitor (open circles). (e) RHC80267 concentration–inhibition curve (IC50 = 9 ± 1 μM; n = 7) against Ca2+ responses evoked by CCL2 (50 ng·ml−1). (f) Effect of 30‐μM RHC80267 on CCL2 concentration–response curve (n = 7). (g) Effect of R59949 (30 μM) and RHC80267 (30 μM) on THP‐1 transmigration to CCL2 (3 ng·ml−1). *P < .05 versus vehicle and # P < .05 versus CCL2 alone (n = 8). F ratio is the Ca2+ response as measured by the Fura‐2 emission intensity ratio when excited at 340 and 380 nm. Data in concentration–response/inhibition curves are expressed as a percentage of the control response in the presence of vehicle alone. (h) Biochemical measurement of DAG changes in THP‐1 cells. Cells preincubated for 30 min with U73122 (5 μM), R59949 (30 μM), or RHC80267 (30 μM) prior to CCL2 challenge (50 ng·ml−1) for 1 or 2 min (n = 6). Vehicle control; cells are preincubated with vehicle and not challenged with CCL2. *P < .05 versus CCL2 alone

Importantly, inhibiting DAG kinase and DAG lipase attenuated CCL2‐evoked signalling in freshly isolated human CD14+ monocytes (Figure 3). R59949 (30 μM; Figure 3a) and RHC80267 (30 μM; Figure 3b) inhibited CCL2‐evoked Ca2+ signals, inhibiting the peak Ca2+ response by approximately 75% and 30% (Figure 3c), respectively. Furthermore, inhibiting both DAG kinase and DAG lipase attenated CCL2‐stimulated migration in freshly isolated monocytes (Figure 3d). Interestingly, intracellular Ca2+ responses elicited as a consequence of activation of the formyl peptide receptor on monocytes with n‐formylmethionine‐leucyl‐phenylalanine (fMLP) was insensitive to either R59949 (Figure 3e) or RHC80267 (Figure 3f), which suggests that neither DAG kinase nor DAG lipase inhibition is a generic regulator of receptor‐mediated Ca2+ signalling in monocytes (Figure 3g). Although the focus of this study is CCL2, we also investigated the effect of R59949 and RHC80267 on CCL5‐mediated responses in freshly isolated monocytes. CCL5 has been reported to activate the chemokine receptors CCR1, CCR3, and CCR5 (de Wit, de Munnik, Leurs, Wischer, & Smit, 2016) and is also implicated in the onset and progression of atherosclerosis (Schober et al., 2002). In monocytes, we observed that CCL5 mediates intracellular Ca2+ response through activation of CCR1, but not CCR3 or CCR5 (Figure S1). The activity of CCR1 is also attenuated following DAG kinase or DAG lipase inhibition. However, the ability of CXCL1, which is implicated in monocyte mobilisation under chronic inflammatory conditions (Drechsler, Duchene, & Soehnlein, 2015), to evoke intracellular Ca2+ responses in monocytes was attenuated by inhibition of DAG kinase but not DAG lipase (Figure S2). In monocytes, we observed that CXCL1‐evoked Ca2+ responses are mediated by CXCR2 activation (Figure S2).

Figure 3.

Figure 3

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Responses to CCL2 but not fMLP are attenuated by DAG kinase and DAG lipase inhibitors in freshly isolated human monocytes. Effect of (a) DAG kinase inhibitor R59949 (30 μM) and (b) DAG lipase inhibitor RHC80267 (30 μM) on Ca2+ responses evoked by CCL2 (50 ng·ml−1) in monocytes (n = 8). Averaged responses are shown in the presence of vehicle (closed circles) and inhibitor (open circles). (c) Bar chart showing effect of R59949 (30 μM) and RHC80267 (30 μM) on the peak Ca2+ response evoked by CCL2 (50 ng·ml−1; n = 8). (d) Effect of R59949 (30 μM) and RHC80267 (30 μM) on freshly isolated monocyte transmigration to CCL2 (3 ng·ml−1). *P < .05 versus vehicle and # P < .05 versus CCL2 alone (n = 8). Lack of effect of (e) R59949 (30 μM) or (f) RHC80267 (30 μM) on Ca2+ responses evoked by fMLP (10 μM) in monocytes (n = 6). Averaged responses are shown in the presence of vehicle (closed circles) and inhibitor (open circles). (g) Bar chart showing lack of effect of R59949 (30 μM) and RHC80267 (30 μM) on peak Ca2+ response evoked by fMLP (10 μM; n = 6). F ratio is the Ca2+ response as measured by the Fura‐2 emission intensity ratio when excited at 340 and 380 nm. Data in inhibition experiments are expressed as a percentage of the control response in the presence of vehicle alone

Next, we profiled the expression of DAG kinase and DAG lipase isoforms expressed in freshly isolated human CD14+ monocytes and THP‐1 monocytic cells. RT‐PCR analysis of mRNA transcripts revealed an overlapping expression profile of DAG kinase and DAG lipase isoforms in CD14+ monocytes and THP‐1 cells (Table 1). For DAG kinase isoforms, α, γ, δ, η, ε, θ, κ, and ζ were expressed by both cell types, and β and ι were not. For DAG lipase isoforms, isoforms α and β were expressed by CD14+ monocytes and THP‐1 cells (Table 1). To corroborate these findings, we confirmed expression at the protein level by immunocytochemistry in THP‐1 cells (Figure S3).

3.2. The amount of cell surface CCR2 is unaffected by DAG kinase or DAG lipase inhibition

A possible mechanism underlying the reduced responsivity to CCL2 following inhibition of DAG metabolism is a reduction in the number of cell surface CCR2 receptors. To test this hypothesis, we quantified CCR2 cell surface expression in freshly isolated monocytes and THP‐1 cells following R59949 or RHC80267 treatment by flow cytometry. A PE‐conjugated antibody recognising human CCR2 labelled CCR2 CD14+ monocytes (Figure 4a) and THP‐1 cells (Figure 4b) over an isotype control. R59949 and RHC80267 were applied to cells to mimic the protocol used to investigating Ca2+ signalling. Despite this, neither R59949 nor RHC80267 had any significant effect on CCR2 cell surface expression in THP‐1 cells or human CD14+ monocytes (Figure 4).

Figure 4.

Figure 4

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Inhibition of DAG kinase or DAG lipase does not reduce the cell surface population of CCR2 in freshly isolated monocytes and THP‐1 cells. Three representative (n = 6) flow cytometry profiles of freshly isolated CD14+ monocytes (a) and THP‐1 cells (b) labelled with anti‐CCR2 antibodies or isotype control. Cells were treated with vehicle control, R59949 (30 μM), or RHC80267 (30 μM). Anti‐CCR2 cell surface immunoreactivity is indistinguishable between vehicle control and test groups

To further understand the role of DAG kinase and DAG lipase activity in shaping CCL2‐evoked intracellular Ca2+ responses, we examined the effect of the inhibitors on the responses in the absence of extracellular Ca2+ to negate Ca2+ entry. Under these conditions, CCL2 evoked a rapidly rising but transient Ca2+ response which returned to baseline (Figure 5a). DAG kinase inhibition with R5549 attenuated the peak response but lead to a sustained plateau phase after the transient response (Figure 5a,b), exemplified by an increased AUC (Figure 5c). Unlike DAG kinase inhibition, DAG lipase inhibition with RHC80267 did not affect the transient phase (Figure 5d,e) but did lead to a sustained plateau phase after the transient response (Figure 5f). The AUC for CCL2‐evoked responses under conditions of no external Ca2+ was significantly large following DAG lipase inhibition compared to DAG kinase inhibition, reflecting the difference in degree of inhibition observed in conditions with external Ca2+ (Figure 2). These data suggest that although both DAG kinase inhibition and DAG lipase inhibition suppress the global Ca2+ response to CCL2, they may do so via different mechanisms.

Figure 5.

Figure 5

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Effects of DAG kinase and DAG lipase inhibitors on CCL2‐evoked Ca2+ responses in THP‐1 cells in the absence of extracellular Ca2+. (a) Averaged (n = 8) intracellular Ca2+ responses evoked by CCL2 (50 ng·ml−1) in the absence of extracellular Ca2+ and presence (open circles) and absence (closed circles) of R59949 (30 μM). (b) and (c) show the effect of R59949 on intracellular Ca2+ peak and AUC in the absence of extracellular Ca2+ (n = 8). (d) Averaged (n = 8) intracellular Ca2+ responses evoked by CCL2 (50 ng·ml−1) in the absence of extracellular Ca2+ and presence (open circles) and absence (closed circles) of RHC80267 (30 μM). (e) and (f) show the effect of R59949 on intracellular Ca2+ peak and AUC in the absence of extracellular Ca2+ (n = 8). *P < .05 versus vehicle control for all

3.3. Attenuating effect of DAG metabolism inhibitors is mimicked by 1‐oleoyl‐2‐acetyl‐sn‐glycerol but not rescued by phosphatidylinositol 4,5‐bisphosphate

Following receptor‐mediated hydrolysis of PIP2 to DAG and IP3, DAG is used as a substrate for the rapid resynthesis of PIP2. We therefore reasoned that limiting DAG metabolism could therefore limit PIP2 resynthesis and reduce the pool of PIP2 available for receptor‐mediated hydrolysis, this in time could underlie the attenuated CCL2‐mediated Ca2+ response observed. To this end, we attempted to reverse the effect of DAG kinase inhibition by supplementing cells with exogenous PIP2 (Kantonen et al., 2011). However, in these experiments, exogenous PIP2 did not limit the ability of R59949 to suppress CCL2‐evoked Ca2+ signals (Figures 6a,b), suggesting that PIP2 availability did not underlie the inhibition. We therefore attempted to address whether the accumulation of DAG itself following pharmacological inhibition of its metabolism could mediate the attenuation of Ca2+ signalling. We observed that 1‐oleoyl‐2‐acetyl‐sn‐glycerol (OAG), a membrane permeable DAG analogue (Assani et al., 2017), could mimic the effect of DAG kinase inhibition or DAG lipase inhibition (Figure 6c) and inhibit CCL2‐evoked Ca2+ signalling in a concentration fashion (Figure 6d). The half‐maximal concentration for OAG was 9.2 ± 1.2 μM (n = 6), and the maximum CCL2 response was suppressed by approximately 70% at 30‐μM OAG (Figure 6e).

Figure 6.

Figure 6

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Application of exogenous PIP2 does not rescue CCL2‐evoked Ca2+ response following DAG kinase inhibition, but inhibition is mimicked by OAG in THP‐1 cells. (a) CCL2‐evoked (50 ng·ml−1) intracellular Ca2+ responses in the presence of vehicle control (closed circles), R59949 (open circles; 30 μM), or R59949 plus exogenous PIP2 (squares; 300 μM; n = 8). (b) Bar chart showing average peak intracellular Ca2+ responses. *P < .05 versus vehicle control. (c) CCL2‐evoked (50 ng·ml−1) intracellular Ca2+ responses in the presence of vehicle control (closed circles) or cell permeable DAG analogue, OAG (open circles; n = 8). (d) Concentration–inhibition curve for OAG effect on intracellular Ca2+ responses evoked by CCL2 (50 ng·ml−1; n = 8). (e) Effect of OAG (30 μM) on CCL2 concentration–response curve in THP‐1 cells (IC50 9 ± 1 μM; n = 6). Responses are in the presence of vehicle control (closed circles) or OAG (open circles). F ratio is the Ca2+ response as measured by the Fura‐2 emission intensity ratio when excited at 340 and 380 nm. Data in inhibition experiments are expressed as a percentage of the control response in the presence of vehicle alone

3.4. Differential dependency on PKC for effects of DAG metabolism inhibitors and OAG

As DAG is a well‐characterised activator of PKC, we sought to test whether PKC activity was required for the suppressive action of OAG, DAG kinase inhibition, and DAG lipase inhibition. RT‐PCR analysis of PKC isoform mRNA transcripts revealed expression of α, β, δ, η, ε, θ, ι, and ζ but not γ in THP‐1 cells (Table 1). We confirmed the expression of PKCα by immunocytochemistry (Figure S3). The expression pattern was the same in freshly isolated CD14+ monocytes except that PKCε was not expressed (Table 1). Due to the diverse repertoire of PKC isoforms expressed, we employed pharmacological tools that allowed discrimination between classical DAG and Ca2+‐dependent isoforms (α, β, and γ; blocked by Gö6976) and DAG dependent but Ca2+‐independent isoforms (δ, ε, η, or θ; blocked by Gö6983); Gö6983 also blocks α, β, and γ isoforms (Goekjian & Jirousek, 1999; Gschwendt et al., 1996). Gö6983 100‐nM (Young, Rey, Sinnett‐Smith, & Rozengurt, 2014) had no effect on the control Ca2+ response to CCL2 (Figure 7a); however, 100‐nM Gö6976 (Lin, Leu, Huang, & Tsai, 2011) significantly inhibited the response (Figure 7a). Gö6983 could rescue the response inhibited by OAG (Figure 7b), R59949 (Figure 7c), or RHC80267 (Figure 7d), though Gö6976 could not (Figure 7b–d). These data, summarised in Figure 7e, suggest that the inhibitory action of exogenous DAG (OAG) on DAG metabolism is mediated via a Ca2+‐independent PKC isoform. The inhibitory action of R59949 and RHC80267 on CCL2‐evoked Ca2+ in freshly isolated monocytes could also be reversed by Gö6983 (n = 5; Figure 7f).

Figure 7.

Figure 7

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Effect of inhibiting Ca2+‐dependent and Ca2+‐independent PKC isoforms on CCL2‐evoked responses following inhibition of DAG kinase and DAG lipase in THP‐1 cells and freshly isolated monocytes. (a) CCL2‐evoked intracellular Ca2+ responses in THP‐1 cells in the presence of vehicle control, Gö6976 (100 nM), or Gö6983 (100 nM; n = 8). (b) CCL2‐evoked intracellular Ca2+ responses in THP‐1 cells in the presence of vehicle control and OAG (30 μM) in the presence and absence of Gö6976 or Gö6983 (n = 8). (c) CCL2‐evoked intracellular Ca2+ responses in THP‐1 cells in the presence of vehicle control and R59949 (30 μM) in the presence and absence of Gö6976 or Gö6983 (n = 8). (d) CCL2‐evoked intracellular Ca2+ responses in THP‐1 cells in the presence of vehicle control and RHC80267 (30 μM) in the presence and absence of Gö6976 or Gö6983 (n = 8). (e) Bar chart showing averaged data from experiments (a–d). (f) Bar chart showing CCL2‐evoked Ca2+ responses in freshly isolated monocytes and the effect of R59949 (30 μM) and RHC80267 (30 μM), in the presence and absence of Gö6983 (100 nM; n = 8). All intracellular Ca2+ responses were evoked by 50‐ng·ml−1 CCL2. *P < .05 versus CCL2 and # P < .05 for combined inhibitors compared to OAG, R59949, or RHC80267 alone. F ratio is the Ca2+ response as measured by the Fura‐2 emission intensity ratio when excited at 340 and 380 nm. Data in inhibition experiments are expressed as a percentage of the control response in the presence of vehicle alone

3.5. The Ca2+‐sensitive isoform PKCα regulates CCL2‐evoked Ca2+ signalling in THP‐1 cells

A striking observation of the experiments with Gö6976 was its ability to inhibit CCL2‐evoked Ca2+ signalling without pharmacological manipulation of DAG metabolism. These data suggest that a DAG and Ca2+‐dependent PKC isoform may regulate the CCL2 response, and to investigate this further, we attempted siRNA‐mediated knock‐down studies of the classical Ca2+‐sensitive PKC isoform PKCα. In these experiments, siRNA delivery to THP‐1 monocytes could inhibit CCL2‐evoked Ca2+ responses versus scrambled siRNA counterparts (Figure 8a). Though the response peak was unaffected (Figure 8b), PKCα knock‐down significantly reduced response AUC (Figure 8c). Quantitative RT‐PCR confirmed PKCα mRNA knock‐down of approximately 50% versus scrambled siRNA counterparts (Figure 8d). These data suggest that the activity of PKCα is required for THP‐1 cells to respond to CCL2 at control levels.

Figure 8.

Figure 8

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Effect of DAG kinase α knock‐down of CCL2‐evoked Ca2+ responses in THP‐1 cells. (a) Averaged intracellular Ca2+ response evoked by CCL2 in THP‐1 cells transfected with scrambled siRNA (closed circles) or DAG kinase α targeted siRNA (open circles; n = 8). Bar charts showing peak (b) and AUC (c) intracellular Ca2+ responses evoked by CCL2 in scrambled, GAPDH knock‐down, or DAG kinase α knock‐down THP‐1 cells (n = 8). (d) qRT‐PCR analysis of GAPDH or DAG kinase α mRNA transcripts in scrambled and knock‐down THP‐1 cells (n = 8). F ratio is the Ca2+ response as measured by the Fura‐2 emission intensity ratio when excited at 340 and 380 nm. Responses evoked by 50‐ng·ml−1 CCL2 for all experiments. *P < .05 versus scrambled control cells in all experiments. Data in each experiment are expressed as a percentage of the Ca2+ response evoked by ionomycin in control for cell number in knock‐down studies

LDH release assays were performed to test for potential cytotoxic effects of inhibitor treatments applied throughout the study (Figure S4).

4. DISCUSSION

This study reconfirms that CCR2 is the cognate receptor for CCL2 in human CD14+ monocytes and THP‐1 cells. We also provide molecular and function evidence that both DAG kinase and DAG lipase are functional routes for the metabolism of DAG arising from receptor‐mediated DAG production. These results corroborate studies in T‐lymphocytes (Lee, Kim, Beste, Korestzky, & Hammer, 2012) and cancer cells (Rainero et al., 2014) that demonstrate a role for DAG kinases in modulating chemokine functionality. Our data also reveal that CCL5 signalling via CCR1 is regulated by both DAG kinase activity and DAG lipase activity, though lack of effect of DAG lipase inhibition on CXCL1–CXCR2 signalling is suggestive that this mechanism cannot be generalised for all chemokine action at monocytes.

The data suggest that inhibitors of both DAG kinase and DAG lipase are effective in reducing the efficacy of CCL2 signalling in monocytes, as the response maxima are significantly attenuated with little change in CCL2 EC50 values. As the effects of DAG kinase inhibition and DAG lipase inhibition are mimicked by OAG and not rescued by addition of exogenous PIP2, the effect on CCL2 signalling of inhibiting DAG metabolism is likely to be due to the accumulation of DAG rather than limitation of a DAG metabolite or PIP2 synthesis. If this is the case, the data suggest that there is no redundancy between kinase‐ or lipase‐dependent metabolic pathways for DAG in human monocytes and processes that modulate the activity of these enzymes have the potential to modulate CCL2 signalling efficacy. Although CCR2 receptors are classical GPCRs and can undergo internalisation as part of mechanisms of receptor desensitisation (Dzenko, Andjelkovic, Kuziel, & Pachter, 2001; Volpe et al., 2012), the data presented here suggest that the mechanism via which inhibition of DAG metabolism causes loss of CCL2 signalling efficacy is not via a reduction in the cell surface population of CCR2 receptors. This therefore suggests that the inhibitory mechanism must involve modulation of the CCR2 receptor itself, an auxiliary subunit or a downstream effector protein. As the effects of OAG, DAG kinase inhibition, and DAG lipase inhibition are reversed by the broadspectrum PKC inhibitor Gö6983 but not Gö6976, a selective inhibitor of Ca2+‐dependent PKC isoforms, this suggests that the inhibitor effects of DAG accumulation are mediated by a Ca2+‐independent PKC isoform. Analysis of PKC isoform expression suggests that PKCδ, PKCε, PKCη, PKCθ, and PKCζ are potential effectors of the inhibitory actions of DAG in monocytes. Previous studies in monocytes have documented translocation of both Ca2+‐dependent and Ca2+‐independent PKC isoforms from the cytoplasm to the plasma membrane upon stimulation with CCL2 (Zhang, Hodge, Rogers, & Oppenheim, 2003). However, opioid receptor activation, which inhibits CCL2 signalling via heterologous desensitisation, causes membrane recruitment of only Ca2+‐independent PKC isoforms (Zhang et al., 2003). Such studies support a role for Ca2+‐independent PKC isoforms as negative regulators of CCR2 receptor activity. The target of PKC is unlikely to be the CCR2 receptor itself as consensus sequences for PKC‐dependent phosphorylation are absent from the cytoplasmic sections of the receptors, although other chemokine receptors, such as CXCR4, are phosphorylated directly by PKC (Luo, Busillo, Stumm, & Benovic, 2017).

The intracellular Ca2+ signal generated following CCR2 activation in monocytes most likely involves direct release of Ca2+ from ER stores but also Ca2+ through plasma membrane channels (Nardelli et al., 1999). Experiments in the absence of extracellular Ca2+ support this as CCL2 can still elicit a response though transient and lacking a substantial plateau phase. The shape of the intracellular Ca2+ response is also differentially modulated by DAG kinase and DAG lipase inhibitors when the possibility of Ca2+ influx is negated. Both R59949 and RHC80267 elevate the plateau phase of release, but only R59949 inhibits the peak Ca2+ response in the absence of extracellular Ca2+. This suggests that there may be some discrimination regarding how DAG elevation, directly or indirectly, regulates the ability of CCR2 to release stored Ca2+ (Bartlett, Metzger, Gaspers, & Thomas, 2015). Monocytes express a large repertoire of DAG kinase isoforms, and as R59949 is a pan DAG kinase inhibitor, we cannot determine whether redundancy exists between isoforms or whether only some subtypes participate in the regulation of CCR2 activity. siRNA‐mediated knock‐down studies reveal DAG kinase α as a candidate, at least in THP‐1 cells. DAG kinase α has been implicated previously in immune cell function (Sanjuan et al., 2003).

In summary, we demonstrate that inhibition of DAG kinase and DAG lipase is a novel pharmacological route to suppress CCL2‐mediated intracellular Ca2+ signalling and migration in human monocytes. We suggest that the underlying mechanism involves DAG accumulation and activation of Ca2+‐independent PKC isoforms.

CONFLICT OF INTEREST

The authors declare no conflicts of interest.

AUTHOR CONTRIBUTIONS

P.D., L.B., and D.R. carried out the experiments and analysed the data. S.J.F. designed the experiments and wrote the manuscript.

DECLARATION OF TRANSPARENCY AND SCIENTIFIC RIGOUR

This Declaration acknowledges that this paper adheres to the principles for transparent reporting and scientific rigour of preclinical research as stated in the BJP guidelines for Design & Analysis, and Immunoblotting and Immunochemistry, and as recommended by funding agencies, publishers, and other organisations engaged with supporting research.

Supporting information

Figure S1 Effect of DAG kinase and DAG lipase inhibition on CCL5‐evoked response in CD14+ human monocytes.

Figure S2 Effect of DAG kinase and DAG lipase inhibition on CXCL1‐evoked response in CD14+ human monocytes.

Figure S3 Immunocytochemical analysis of DAG kinase and DAG lipase isoform expression in THP‐1 cells.

Figure S4 Compound cytotoxicity assay Cell viability as tested by lactate dehydrogenase (LDH) release.

Click here for additional data file. (1.8MB, pdf)

ACKNOWLEDGEMENT

This work was supported by the British Heart Foundation (PG/16/94/32393).

Day P, Burrows L, Richards D, Fountain SJ. Inhibitors of DAG metabolism suppress CCR2 signalling in human monocytes. Br J Pharmacol. 2019;176:2736–2749. 10.1111/bph.14695

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Associated Data

This section collects any data citations, data availability statements, or supplementary materials included in this article.

Supplementary Materials

Figure S1 Effect of DAG kinase and DAG lipase inhibition on CCL5‐evoked response in CD14+ human monocytes.

Figure S2 Effect of DAG kinase and DAG lipase inhibition on CXCL1‐evoked response in CD14+ human monocytes.

Figure S3 Immunocytochemical analysis of DAG kinase and DAG lipase isoform expression in THP‐1 cells.

Figure S4 Compound cytotoxicity assay Cell viability as tested by lactate dehydrogenase (LDH) release.

Click here for additional data file. (1.8MB, pdf)

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