Morphine tolerance is attenuated in germfree mice and reversed by probiotics, implicating the role of gut microbiome

Morphine Tolerance Was Attenuated in Germfree and Pan-Antibiotics Mice.

We have previously shown that chronic morphine treatment results in microbial dysbiosis, disruption in gut barrier function, and bacterial translocation, primarily through the μ-opioid receptor (OPRM1) (21). To initially establish the role of the gut microbiota in morphine tolerance, germfree (GF) mice and conventionally raised, specific pathogen-free (SPF) mice were subjected to a well-established tolerance regimen wherein mice were treated with either saline or repeated escalating doses of morphine for 8 d. Interestingly, morphine-treated GF mice displayed less analgesic tolerance in both tail flick and hot plate tests than SPF mice, 75% and 25% maximum possible effect (%MPE), respectively (Fig. 1 A and B). We next repeated this experiment in GF mice that had undergone fecal microbiota transplantation (FMT) with samples obtained from SPF mice. These mice showed significant analgesic tolerance similar to SPF animals treated with morphine (Fig. 1 C and D). These results clearly establish the role of gut microbiota in morphine analgesic tolerance.

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Fig. 1.

Gut microbiota are essential for morphine analgesic tolerance. (A and B) Antinociceptive tolerance was attenuated in GF mice. F_{tail flick} (3, 10) = 869.4, and F_{hot plate} (3, 10) = 110.9. (C and D) GF mice recapitulated morphine tolerance after FMT with naïve mouse microbiota. F_{tail flick} (3, 10) = 882.8, and F_{hot plate} (3, 10) = 147.8; n_SPF = 4; n_GF = 3. (E and F) Mice exhibited attenuated analgesic tolerance after gut microbiota depletion; n = 12 to 20. F_{tail flick} (3, 56) = 118.8, and F_{hot plate} (3, 56) = 58.19. (A–F) Data were analyzed by one-way ANOVA followed by Bonferroni correction. **P < 0.01; ****P < 0.0001. (G and H) Time course of the effects of different microbiota on morphine tolerance; n = 6 to 8. F_{Treatment x time} (56, 343) = 73.15 for tail flick. F_{Treatment x time} (56, 343) = 59.66 for hot plate. Two-way ANOVA followed by Tukey’s multiple comparison was used. *P < 0.05; **P < 0.01; ***P < 0.001; ****P < 0.0001 for Morphine vs. Saline microbiome + Morphine. *P < 0.05; **P < 0.01; ***P < 0.001; ****P < 0.0001 for Morphine vs. Morphine microbiome + Morphine. Each dot represents one mouse. Mean ± SD.

To further investigate whether gut microbial dysbiosis contributed to morphine tolerance, SPF mice were administered a mixture of antibiotics in their drinking water for a week to deplete the gut microbiota and then treated with escalating doses of morphine for 8 d. Pan-antibiotics (ABX) treatment was maintained during the whole duration of morphine treatment. Results from these studies show that ABX markedly reduced gut bacteria (SI Appendix, Fig. S1 A and B). ABX and SPF mice were treated with repeated escalating doses of morphine. The morphine-treated ABX mice showed significantly attenuated analgesic tolerance, with 64 %MPE at day 8 in both tail flick and hot plate assays (Fig. 1 E and F). In an additional study, a fixed morphine dose was administered to ABX and SPF control mice twice daily for 8 d. The ABX mice maintained a significantly higher antinociceptive efficacy from day 4 by tail flick (SI Appendix, Fig. S1C) and from day 5 by hot plate (SI Appendix, Fig. S1D) compared with non−antibiotic-treated mice.

To further establish the role of gut microbiota in analgesic tolerance, SPF mice treated with ABX were gavaged with microbiota harvested from either saline- or morphine-treated mice. Mice reconstituted with morphine-tolerant mouse microbiota and then treated with morphine showed exacerbated analgesic tolerance following the same daily injection doses. In contrast, mice that were reconstituted with saline-treated mouse microbiota displayed less analgesic tolerance (Fig. 1 G and H). To validate effective reconstitution, stool samples were collected from recipient mice and subjected to 16S ribosomal RNA (rRNA) sequencing. The microbiome of the recipient animals was similar to their donor profile in principal coordinates analysis clustering (SI Appendix, Fig. S1E). In summary, the data from these studies clearly support a role for gut microbiota in morphine-induced analgesic tolerance.

Morphine-Induced Dysbiosis Disrupted Gut Epithelial Barrier and Promoted Systemic Bacterial Translocation.

We evaluated gut barrier permeability and bacterial translocation in the mice to determine how morphine-induced microbial dysbiosis contributes to analgesic tolerance. Ileum samples were examined for histopathological changes. In SPF morphine-tolerant mice, we observed impaired epithelia and increased inflammatory infiltrates in small intestinal villi (Fig. 2 A, ii). In contrast, in morphine-treated GF and ABX mice, no morphological damage was observed (Fig. 2 A, iv and vi). Morphine-induced intestinal disruption was also seen in GF mice that received naïve microbiota from SPF mice (Fig. 2 B, ii). In the GF or ABX mice undergoing FMT from saline- or morphine-tolerant mice, we observed that FMT from morphine-tolerant mice alone is sufficient to induce histopathological change in the gut, without requiring direct exposure to morphine (Fig. 2 C, ii and iv). To evaluate the disruption in gut permeability, SPF and ABX mice with or without FMT were gavaged with fluorescein isothiocyanate (FITC)-dextran. Significant increase in gut permeability was observed in SPF morphine-tolerant mice (Fig. 2D). Morphine’s effects on gut permeability of SPF mice were abolished in ABX-treated mice (Fig. 2D). In ABX mice that underwent FMT, a significant increase in FITC-dextran in the serum was observed in the mice receiving gut microbiota from morphine-tolerant mice (Fig. 2E), but not in those receiving gut microbiota from saline-treated mice. We next evaluated gut bacterial translocation to the liver and mesenteric lymph nodes (MLN) in the mice. Significant bacterial translocation was observed in SPF morphine-tolerant mice (Fig. 2F and SI Appendix, Fig. S2A). As expected, morphine treatment failed to induce bacterial translocation in either GF or ABX mice (Fig. 2F and SI Appendix, Fig. S2A). However, when GF mice were reconstituted with the microbiota of naïve SPF mice, and then treated with morphine, bacterial translocation was observed (Fig. 2G and SI Appendix, Fig. S2B). In addition, when GF mice or ABX mice underwent FMT, the mice receiving morphine-tolerant microbiota showed significantly greater bacterial translocation than the mice receiving microbiota of saline-treated animals (Fig. 2H and SI Appendix, Fig. S2C). These studies suggest that morphine-induced gut integrity disruption and subsequent bacterial translocation is mediated by alterations in the gut microbiota. These results provide further evidence for the crucial role of morphine-induced dysbiosis in analgesic tolerance.

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Fig. 2.

Gut microbiome is responsible for gut permeability and bacterial translocation induced by morphine. (A–C) Representative H&E stained section of mouse ileum. (Scale bar: 100 μm.) WT and ABX mice: n_SPF = 10, n_GF = 3. (D and E) Representative images and summary of FITC-dextran fluorescent signal distribution in mice; n = 6 to 11. (F) Bacterial colony-forming unit (CFU) in liver homogenates of GF and SPF mice; n_SPF = 10 to 20; n_GF = 3. Data were analyzed by one-way ANOVA followed by Bonferroni’s multiple comparisons test. (G) CFU from GF mice reconstituted with normal gut microbiota and treated with either morphine or saline; n_GF = 3. (H) CFU from GF mice and ABX-treated SPF mice received gut microbiota either from saline or morphine-tolerant donors; n_GF = 3; n_SPF/ABX = 10 to 12. Data were analyzed by Student’s t test. *P < 0.05; **P < 0.01; ***P < 0.001; ****P < 0.0001. Mean ± SD.

Morphine-Tolerant Animals Displayed Higher Expression of TLR2 and TLR4.

To further explore the characteristics of the translocated bacteria in the liver and MLN, we analyzed DNA isolated from the liver by gel-based PCR using the primers specific for Gram-positive and Gram-negative bacteria. We found both Gram-positive and Gram-negative bacteria translocating to the liver in the morphine-tolerant animals (SI Appendix, Fig. S3 A and B). TLR2 and TLR4 are the major receptors that mediate the host’s response to Gram-positive and Gram-negative bacteria, respectively. To determine the roles of TLR2 and TLR4 in morphine analgesic tolerance, we evaluated expression of these receptors on gut epithelial and immune cells. In morphine-tolerant animals, we found a significant increase in TLR2 and TLR4 expression in both gut epithelial cells (Fig. 3A and SI Appendix, Figs. S3C and S4A) and intraepithelial immune cells (Fig. 3B and SI Appendix, Figs. S3D and S4B). Furthermore, the expression of TLR2 and TLR4 was also significantly increased in circulating immune cells isolated from the blood of morphine-tolerant animals (Fig. 3C and SI Appendix, Figs. S3E and S4C). The expression levels of TLR2 and TLR4 were not up-regulated by morphine treatment in ABX mice (Fig. 3 A and B and SI Appendix, Fig. S3 C and D). Surprisingly, in circulating immune cells, morphine increased TLR4 expression in GF mice (SI Appendix, Fig. S4C). However, in ABX mice, TLR4 expression on circulating immune cells was not elevated by morphine (SI Appendix, Fig. S4C). After reconstituting the GF mice with the naïve microbiome of SPF mice, morphine treatment induced tolerance in these mice, and elevated TLR2 and TLR4 expression on gut epithelial and immune cells (Fig. 3 D–F and SI Appendix, Figs. S3 F–H and S4 D–F). Moreover, transplantation of microbiota from morphine-tolerant mice alone was sufficient to enhance TLR2 and TLR4 protein expression in GF and ABX mice (Fig. 3 G–I and SI Appendix, Figs. S3 I–K and S4 G–I). These data suggest that TLR2 and TLR4 activation, as a consequence of dysbiosis and bacterial translocation, and the resulting induction of proinflammatory cytokines may be mediators of morphine analgesic tolerance. To further delineate the roles of TLR2 and TLR4 in morphine analgesic tolerance, TLR2 and TLR4 Knockout (TLR2KO and TLR4KO) mice were treated with repeated injections of morphine [either with escalated (Fig. 3 J and K) or fixed doses (SI Appendix, Fig. S3 L and M)]. We found that morphine-induced analgesic tolerance was partially attenuated in both TLR2KO and TLR4KO mice using either tail flick (Fig. 3J) or hot plate (Fig. 3K) assays. Although morphine-induced analgesic tolerance was modulated by both TLR2 and TLR4, it was more significantly attenuated in TLR2KO mice (Fig. 3 J and K), with reduced gut barrier disruption (Fig. 3L) and lower bacterial translocation (Fig. 3M). This suggests a more important role for TLR2 in morphine analgesic tolerance.

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Fig. 3.

Morphine regulates gut and systemic TLR2 expression through gut microbiome. (A−C) The up-regulation of TLR2 expression by morphine was suppressed in GF and ABX mice; n_GF = 3; n_SPF = 12 to 15. (D−F) Morphine induced TLR2 expression in GF mice following gavaging with naïve mouse microbiota; n_GF = 3. (A–F) Data were analyzed by one-way ANOVA followed by Bonferroni’s multiple comparisons test. (G−I) The microbiota FMT from morphine-tolerant mice alone increased TLR2 expression in GF and ABX mice; n_GF = 3; n_ABX = 5. Two-tailed Student’s t test was used for statistical analysis. (J and K) Morphine analgesic tolerance was determined in WT, TLR2KO, and TLR4KO mice. F_{tail flick} (5, 46) = 75.71; F_{hot plate} (5, 46) = 42.04; n = 8 to 10. (L) (i) Representative images and (ii) summary of fluorescent signal distribution in morphine-treated WT, TLR2KO, and TLR4KO mice; n = 6 to 10. (M) Visualization of bacterial colonies in blood agar plates from liver homogenates. (J–M) One-way ANOVA followed by Bonferroni’s multiple comparisons test was used for statistical analysis. *P < 0.05; **P < 0.01; ***P < 0.001; ****P < 0.0001. Mean ± SD.

Morphine-Tolerant Animals Displayed Sustained Chronic Systemic Inflammation.

Accumulating evidence implicates inflammation as a contributing factor in morphine-induced analgesic tolerance. To further investigate the role of inflammatory cytokines in this process, animals were subjected to repeated morphine injections. In morphine-tolerant animals, the protein levels of proinflammatory cytokines IL-6, IL-1β, and TNF-α were measured in the liver, MLN, and brain by enzyme-linked immunosorbent assay (ELISA). Additionally, messenger RNA levels of these cytokines were also determined in the spinal cords and intestines. Morphine-tolerant animals displayed significantly elevated levels of these cytokines in all tissues examined. However, morphine administration to GF and ABX mice showed less inflammatory response (Fig. 4 A and B and SI Appendix, Table S1 and Fig. S5 A, B, I, and J). GF mice receiving naïve SPF microbiota developed analgesic tolerance and displayed higher expressions of these cytokines following morphine treatment (Fig. 4 C and D and SI Appendix, Table S2 and Fig. S5 C, D, K, and L). FMT of the gut microbiota from morphine-tolerant mice into GF and ABX recipients resulted in increased expression of these cytokines (Fig. 4 E and F and SI Appendix, Table S3 and Fig. S5 E, F, M, and N). Repeated morphine injections into TLR2KO and TLR4KO mice, as previously mentioned, induced less inflammation than equivalent injections into WT mice (Fig. 4 G and H and SI Appendix, Table S4 and Figs. S4 G and H and S5 G, H, O, and P). Together, these studies demonstrate that alteration in microbial compositions disrupted gut integrity, facilitated bacterial translocation, regulated TLR expressions and activation, and exacerbated inflammation, all contributing to morphine tolerance. Since morphine-tolerant animals showed a significant increase in IL-6 protein levels, we hypothesized that IL-6 may be one of the mediators of morphine tolerance. To test this hypothesis, IL-6 Knockout (IL-6KO) mice were subjected to repeated morphine injections to induce analgesic tolerance. Analgesic tolerance for both tail flick (30.23 %MPE vs. 42.82 %MPE) and hot plate assays (23.44 %MPE vs. 35.89 %MPE) (Fig. 4 I and J and SI Appendix, Fig. S5 Q and R) were only partially attenuated in these mice, indicating that other proinflammatory cytokines may also contribute to modulating analgesic tolerance. Gut histological damage (SI Appendix, Fig. S5U) and bacterial translocation (SI Appendix, Fig. S5 S and T) were also attenuated in IL-6KO mice.

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Fig. 4.

Gut microbiome is essential for morphine-induced chronic systemic inflammation. (A and B) IL-6 expression in morphine-treated GF and ABX mice was reduced compared with WT controls; n_GF = 3; n_SPF = 10 to 17. (C and D) Morphine effect on IL-6 expression was restored after gut microbiota was reconstituted in GF mice; n_GF = 3. (A–D) Data were analyzed using one-way ANOVA followed by Bonferroni’s multiple comparisons test. (E and F) GF and ABX mice were gavaged with microbiota from either saline or morphine-tolerant mice; n_GF = 3; n_SPF/ABX = 13 to 15. Significance was tested by two-tailed Student’s t test. (G and H) IL-6 expression was detected in WT, TLR2KO, and TLR4KO mice; n = 8 to 16. (I and J) WT and IL-6KO mice were treated with escalating morphine dosing for 8 d; n = 13 to 17. F_{tail flick} (3, 56) = 206.1. F_{hot plate} (3, 56) = 268.9. Data were analyzed by one-way ANOVA followed by Bonferroni’s multiple comparisons test. *P < 0.05; **P < 0.01; ***P < 0.001; ****P < 0.0001. Mean ± SD.

Morphine Analgesic Tolerance Resulted in Significant Alterations in Gut Microbiome.

To determine whether microbial dysbiosis contributed to morphine analgesic tolerance, mice were treated with repeated morphine injections to induce analgesic tolerance. On day 8, small intestinal fecal contents were collected from morphine-tolerant mice (WT, TLR2KO, and TLR4KO) and their corresponding saline-treated controls. Fecal DNA was extracted and subjected to 16S rRNA sequencing. β-diversity analysis revealed a distinct clustering of the bacterial communities in the morphine-tolerant animals compared with saline-treated mice (P = 0.00256, permutation ANOVA (PERMANOVA) test with Bonferroni correction) (Fig. 5A). However, in TLR2KO and TLR4KO mice, using the same β-diversity matrix, we found no difference in the bacterial profiles between saline- and morphine-treated groups (P = 0.217, Fig. 5B; P = 0.183, Fig. 5C). Further analysis revealed a reduction in the relative abundance of Actinobacteria and Firmicutes at the phylum level in morphine-tolerant animals (Fig. 5D and Dataset S1). Furthermore, morphine-tolerant animals also displayed a reduction in Bifidobacteriaceae and Lactobacillaceae at the family level and Bifidobacterium and Lactobacillus at the genus level. The changes observed with WT morphine-tolerant animals were not observed in TLR2KO or TLR4KO morphine-treated mice (Fig. 5 E and F). These data imply that the microbiota of TLR2KO and TLR4KO are very stable and resist any change as a consequence of morphine treatment.

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Fig. 5.

Morphine analgesic tolerance induces gut dysbiosis. (A−C) Multidimensional scaling analysis of gut microbiota to visualize the Bray−Curtis distance of WT, TLR2KO, and TLR4KO morphine-tolerant mice and their controls. Red circles depict samples from morphine-tolerant mice; blue triangles represent WT saline-treated mice. β-diversity was found to be significantly different between the WT morphine-tolerant and saline-treated groups (P = 0.00256). (D) Taxonomic distribution of WT, TLR2KO, and TLR4KO morphine-tolerant mice and their controls at phylum level. Each column represents a fecal sample from a treatment group. (E and F) Dot plots show changes in abundance of bacteria with morphine treatment in WT, TLR2KO, and TLR4KO at family and genus level using WT saline mean proportion as reference. Microbial taxa with significant difference in WT mice were selected at false discovery rate < 0.1 and average relative abundance of WT control > 0.1%; n_WT = 6 to 7; n_TLR2KO = 19 to 24; n_TLR4KO = 8 to 11. NMDS, nonmetric multidimensional scaling.

Morphine Analgesic Tolerance Was Attenuated by Treatment with Probiotics.

Our microbial analyses showed that the relative abundance in the Operational Taxonomic Unit representing Lactobacillaceae and Bifidobacteriaceae was significantly reduced in morphine-tolerant animals. To investigate whether supplementation with these beneficial bacteria attenuates morphine tolerance, the mice were gavaged with probiotics VSL#3. We found a dramatic decrease in morphine antinociceptive tolerance with VSL#3 pretreatment compared with sham mice following escalated morphine treatment in both tail flick (34.74 %MPE vs. 54.23 %MPE) and hot plate (30.04 %MPE vs. 51.09 %MPE) (Fig. 6 A and B) tests. Similarly, probiotics pretreatment alleviated morphine tolerance after constant doses of morphine treatment (SI Appendix, Fig. S6 A and B). Measured by β-diversity, probiotics pretreatment decreased morphine-induced microbial alterations, indicating that VSL#3 probiotics restored partial gut microbial components (Fig. 6C) (P = 0.00096 for Water+Morphine and Water+Saline; P = 0.00012 for Water+Morphine and VSL#3+Saline; P = 0.0024 for VSL#3+Morphine and Water+Saline; P = 0.02592 for VSL#3+Morphine and VSL#3+Saline). Notably, bacterial communities that were significantly reduced in relative abundance in morphine-tolerant animals were substantially restored compared with saline control sample (Fig. 6 D–F and Dataset S1). A close observation of gut histology showed less immune cell infiltration and gut epithelial damage in probiotics-treated mice (Fig. 6G). Notably, morphine-induced gut permeability (Fig. 6H) and systemic bacterial translocation into liver and MLN (Fig. 6I and SI Appendix, Fig. S6C) were rescued using probiotics treatment. Furthermore, morphine tolerance induced increases in TLR2 and TLR4 expression on the gut epithelia, gut, and systemic immune cells (Fig. 6 J–L and SI Appendix, Fig. S6 D–F and G−I), and elevated proinflammatory cytokines IL-6 (Fig. 6 M and N and SI Appendix, Table S5), IL-1β (SI Appendix, Fig. S6 J and K), and TNF-α (SI Appendix, Fig. S6 L and M), which were also ameliorated by probiotics pretreatment. These data clearly support the use of probiotics as an adjunct therapy in patients using opioids for pain management.

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Fig. 6.

Probiotics VSL#3 pretreatment attenuates morphine tolerance and prevents morphine-induced gut microbiota alterations. (A and B) Morphine analgesic effect was determined after escalating doses of morphine; n = 10 to 20. F_{tail flick} (3, 51) = 46.78. F_{hot plate} (3, 51) = 82.50. One-way ANOVA followed by Bonferroni’s correction was used to analyze data. (C) Multidimensional scaling was used to visualize the Bray−Curtis distance of different groups; n = 9 to 15. Data were subjected to PERMANOVA test along with Bonferroni correction. (D) Taxonomic distribution of different groups at phylum level. (E and F) Dot plots show changes in abundance of bacteria in Water+Morphine-treated and VSL#3+Morphine-treated mice at family and genus level using Water+Saline mean proportion as reference; n = 9 to 15. (G) Representative H&E stained intestinal sections from different treatment groups; n = 6 to 10. (H) (i) Representative figure of florescent signal distribution and (ii) summary of serum FITC-dextran concentration from different treatment groups; n = 6 to 10. (I) CFU from liver homogenate of each mouse in different treatment groups; n = 6 to 20. (J−L) Probiotics pretreatment inhibits TLR2 up-regulation by morphine on epithelial and immune cells; n = 11 to 14. (M and N) RT-PCR of the IL-6 gene expression; n = 9 to 19. (E–N) The results were analyzed by one-way ANOVA followed by Bonferroni’s multiple comparisons test. *P < 0.05; **P < 0.01; ***P < 0.001; ****P < 0.0001. Mean ± SD.