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The IL-8 luciferase reporter cell line, THP-G8 cells, used in the
Environmental quality monitoring of surface waters is fundamental to the sustainable management of water resources and to reducing risks posed by multiple anthropogenic stressors (Geissen et al., 2015[
Lipopolysaccharides (LPSs), which are the outer membranes of gram-negative bacterial or cyanobacterial cells, are also widely known to cause strong innate immune reactions in humans via Toll-like receptors (TLRs) on the cell surface. LPS are also called endotoxins because of their biological activity (reviewed by Mazgaeen and Gurung, 2020[
On the other hand, in the internationally validated protocol of the MAT, the sample is incubated with fresh or cryopreserved human whole blood, and the proinflammatory cytokine interleukin-1β is detected by enzyme-linked immunosorbent assay. In contrast to the LAL test, it can detect non-lipopolysaccharide toxins, such as lipoteichoic acid, exotoxins and fungal components (Daneshian et al., 2009[
We established an IL-8 reporter cell line, THP-G8, derived from a human monocyte cell line, that harbors stable luciferase orange (SLO) and stable luciferase red (SLR) genes under the control of the IL-8 and G3PDH promoters, respectively (Takahashi et al., 2011[
In contrast to the MAT that quantitatively measures IL-1β secreted by monocytes, the IL-8 luciferase assay using THP-G8 measures the luciferase activity driven by IL-8 promoter. Wang et al. reported by using cDNA array analysis that, in human monocytes, the highest activated genes for proinflammatory mediators induced by bacterial stimulants (
In this study, to develop an
Environmental water around Sendai city was collected on April 6th 2014. It was sunny weather and the highest temperature was 10.2°C. The water was collected at i) Okura dam (northern latitude of 38°19’32”, eastern longitude of 140°42’22”), ii) the midstream of Hirose river (northern latitude of 38°15’56”, eastern longitude of 140°51’18”), iii) the downstream of Natori river (northern latitude of 38°11’59”, eastern longitude of 140°55’5”), iv) Teizan canal (northern latitude of 38°8’13”, eastern longitude of 140°55’57”), and v) Iwanuma sea shore (northern latitude of 38°8’3”, eastern longitude of 140°56’35”). Environmental water around Manila city was collected on December 13th 2012 at i) Pasig river No. 6 (Pas R6; northern latitude of 14°35’37”, eastern longitude of 121°5’31”), ii) Pasig river No. 4 (Pas R4; northern latitude of 14°33’25”, eastern longitude of 121°4’12”), iii) Pasig river No. 2 (Pas R2; northern latitude of 14°35’21”, eastern longitude of 121°0’49”), iv) Paranaque river No. 4 (Par R4; northern latitude of 14°30’14”, eastern longitude of 120°59’39”), v) Paranaque river No. 3 (Par R3; northern latitude of 14°29’53”, eastern longitude of 120°59’37”), and vi) Las Pinas river No. 4 (Las R4; northern latitude of 14°28’30”, eastern longitude of 120°58’33”). The water was collected using 50 mL conical centrifuge tube (Falcon, Corning, NY) and stocked in a -80 °C freezer.
We used THP-G8 cells derived from a human acute monocytic leukemia cell line THP-1 cell line, which contained stable luciferase orange gene (SLO) regulated by IL-8 promoter and stable luciferase red gene (SLR) by G3PDH promoter (Kimura et al., 2015[
Ind-IL8LA = nIL8LA treated with toxins or environmental water/nIL8LA without treatment
%suppression = (1-Ind-IL8LA of THP-G8 cells pretreated with the inhibitor/Ind-IL8LA) x 100.
The collected environmental water was autoclaved for 20 min at 121 °C and 2 atm, and diluted 1000 times with endotoxin free water. Endotoxin level was measured using Toxin SensorTM Chromogenic LAL EndotoxinAssay Kit (GeneScript, Piscataway, NJ) according to the manufacturer’s instructions. To determine the activity of LPS from
The statistically significant induction of Ind-IL8LA by LPS was determined by t-test.
We first examined which TLR or NLR agonists could stimulate nIL8 LA of THP-G8 cells. When THP-G8 cell in 96-well plate were stimulated with agonists of a series of TLRs and NLRs for 6 h, they increased IL8LA by the stimulation with TLR 1, 2, 4, 5, and 6, and NLR 1 and 2 agonists, while GAPLA that reflected cell survival rate did not significantly change (Figure 1
We next determined the minimum concentration of lipopolysaccharides (
Next, we examined the IL8LA of the environmental water at various spots along the rivers around Sendai, Japan and Manila, the Philippines. Although the environmental water from all the spots increased IL8LA at various levels, in general, the level of the IL8LA was lower in the upper stream and higher in the downstream. Namely, IL8LA was slightly augmented by the water from the Okura dam located at the upper stream of Hirose river and from the midstream of Hirose river. On the other hand, it was strongly augmented by the water from the downstream of Natori river and Teizan canal close to the outlet of the river (Figure 3a
We compared the correlation between the endotoxin activity measured by LAL assay and the activity to stimulate IL8LA of the environmental water. There was a significant correlation between them (R2 = 0.8086,
Since THP-G8 cells can respond to a variety of stimuli including electrophiles like haptens, detergents, ROS, several cytokines, and lipopolysaccharide, the environmental water may stimulate THP-G8 cells by xenobiotics and toxins other than LPS. Indeed, the discrepancy between the IL8LA and the endotoxin level of Natori river and Teizan canal suggest the contamination of some substances other than LPS. It is well known that polymyxin B neutralizes the lethal toxicity, limulus gelation activity, and hemodynamic effects of the endotoxin by binding to the lipid A domain, which is the active center of the endotoxin molecule (Morrison and Jacobs, 1976[
We first examined the effects of these inhibitors on IL8LA stimulated with LPS or haptens. The %suppression of polymyxin B and NAC on IL8LA stimulated by LPS was 75.8 and 69.8, respectively. On the other hand, IL8LA stimulated by haptens, methylisothiazolinone and glutaraldehyde, were suppressed by pretreatment of NAC (%suppression=82.0 and 76.2, respectively), but not suppressed by polymyxin B (%suppression=-29.1 and -13.4, respectively). Then we examined their effects on IL8LA stimulated with the environmental water around Sendai and Manila, and the %suppression by polymyxin B and NAC was plotted on X axis and Y axis, respectively (Figure 5
In this study, we first demonstrated that TLR 1, 2, 4, 5, 6, NLR 1 and 2 agonists augmented IL8LA and that LPS dose-dependently stimulated IL8LA with the lowest concentration of 0.03 ng/ml or 0.4 EU/ml. In addition, we have already reported that most of haptens as well as detergents also stimulated IL8LA (Kimura et al., 2015[
THP-G8 can detect LPS at the concentration of higher than 0.03 ng/ml or 0.4 EU/ml (Figure 2
Recently, there are urgent needs for
In contrast to the LAL assay, the IL-8 Luc assay (W) lacks the specificity because it respond to toxins other than LPS and some chemicals. To overcome this problem, we pretreated THP-G8 cells with polymyxin B and NAC. Using these compounds, the IL-8 Luc assay (W) clearly discriminated the increased IL8LA by LPS from that by haptens. Namely, the former was significantly suppressed by both polymyxin B and NAC, while the latter was significantly suppressed only by NAC. Similarly, the environmental water we examined was classified into two group, the polymyxin B high suppression group that mostly consists of the environmental water around Manila and the polymyxin B low suppression group that mainly consists of the environmental water around Sendai. This results suggests that the increased IL8LA by the water from Manila is mostly caused by the contamination of LPS, while that from Japan is at least partially by the contamination of chemicals or toxins other than LPS. This result is just a representative. If the IL-8 Luc assay (W) is combined with other inhibitors, it becomes possible to identify the contaminants that increase IL8LA. This is the third advantage of the IL-8 Luc assay (W) over the LAL assay.
Finally, the procedure of this assay is simple and reproducible. Namely, the culture of THP-G8 cells is relatively easy and does not require the use of trypsin or EDTA. In this assay, the environmental water or chemicals at graded concentrations are added to the wells of a 96-well culture plate. Then, cells adjusted to the optimum concentration are seeded into each well. After 6 h incubation, 100 μl of pre-warmed Tripluc is added to each of the 96 wells. The subsequent process is completely automated. Therefore, the IL-2 Luc assay is a test method that can significantly reduce human error. Moreover, the procedure of the IL-8 Luc assay (W) was almost identical with that of the OECD442E. In other words, the procedure is considered to have been officially validated. This is the fourth advantage of this assay.
Finally, considering the advantage of the IL-8 Luc assay (W) over the gold standard of LAL assay, the IL-8 Luc assay (W) can be used for evaluating the environmental water, even for regulatory purpose.
This work was supported by JSPS KAKENHI (Grant-in-Aid for challenging Exploratory Research, 25550076), Grants-in-Aid from the Ministry of Health, Labor and Welfare (MHLW, 0618010), and Japan Initiative for Global Research Network from Japan Agency for Medical Research and Development (JP19fm010813 and JPwm0125001).
The authors have no conflict of interest to report.