Full Text

Turn on search term navigation

About the Authors:

Zuzanna Rowinska

* E-mail: [email protected]

Affiliations Department of Vascular Surgery and Interdisciplinary Vein Center, St. Josef-Hospital, Ruhr- University Bochum, Bochum, Germany, Institute of Molecular Cardiovascular Research, University Hospital, RWTH Aachen University, Aachen, Germany

ORCID http://orcid.org/0000-0001-8676-0067

Thomas A. Koeppel

Affiliation: Division of Vascular Surgery, Hospital Asklepios St. Georg Hamburg, Hamburg, Germany

Maryam Sanati

Affiliation: Institute of Molecular Cardiovascular Research, University Hospital, RWTH Aachen University, Aachen, Germany

Hubert Schelzig

Affiliation: Department of Vascular and Endovascular Surgery, Düsseldorf University Hospital, Düsseldorf, Germany

Joachim Jankowski

Affiliations Institute of Molecular Cardiovascular Research, University Hospital, RWTH Aachen University, Aachen, Germany, School for Cardiovascular Diseases (CARIM), University of Maastricht, Maastricht, The Netherlands

Christian Weber

Affiliation: Institut for Prevention and Epidemiology of Cardiovascular Disease, Ludwig-Maximilian-University of Munich, Munich, Germany

Alma Zernecke

Contributed equally to this work with: Alma Zernecke, Elisa A. Liehn

Affiliation: Institute of Experimental Biomedicine, University Hospital Würzburg, Würzburg, Germany

Elisa A. Liehn

Contributed equally to this work with: Alma Zernecke, Elisa A. Liehn

Affiliations Institute of Molecular Cardiovascular Research, University Hospital, RWTH Aachen University, Aachen, Germany, Human Genetic Laboratory, University for Medicine and Pharmacy, Craiova, Romania

Introduction

Atherosclerosis is an inflammatory disease of the arteries with a high rate of morbidity and mortality in the Western World. The immune reactions involved in atherosclerotic plaque formation are controlled by lipid mediators, costimulatory molecules and cytokines. Chemokines are a family of chemotactic cytokines that mediate immune cell recruitment and are of high relevance in atherogenesis [1], and targeting of chemokines and their receptors has been shown to reduce experimental atherosclerosis [2–4].

Fractalkine or CX3CL1 is a CX3C chemokine that is expressed in the vessel wall and mediates firm adhesion and chemotaxis of leukocytes expressing its G-protein-coupled receptor, CX3CR1. CX3CL1 is the only member of the CX3C chemokine family and is usually attached to the membrane through a mucin-like domain [5,6].

Fractalkine/CX3CL1 expression has been detected on activated endothelial cells, smooth muscle cells (SMCs), macrophages and platelets, and is involved in the development of numerous inflammatory pathologies including atherosclerosis, rheumatoid arthritis, or graft rejection [7–13]. While the expression of fractalkine and its receptor CX3CR1 is low in healthy vessels, it increases significantly under pathological conditions, such as in atherosclerotic plaques or during allograft rejection [11,13]. In atherosclerotic vessels, its receptor CX3CR1 is expressed on monocytes and tissue resident SMCs. Mice deficient in CX3CR1 (Cx3cr-/- mice) have previously been employed to investigate the function of monocyte survival and recruitment during atherogenesis [14,15]. The CX3CL1-CX3CR1 interaction has been shown to confer essential survival signals in monocytes/macrohages, and absence of CX3CR1 was shown to lead to an increased death of monocytes and/or foam cells, inhibiting atherosclerotic lesion formation [15]. Pharmacological inhibition of the chemokine receptor, CX3CR1 has furthermore been described to inhibit leukocyte recruitment and to reduce atherosclerosis [16], indicating an important role of CX3CL1 in the pathogenesis of atherosclerosis. In addiiton, platelets express CX3CR1, which plays a role in the formation of platelet-monocyte complexes [10]. Moreover, CX3CL1/Fractalkine can elicit chemotactic responses in SMCs and has been described to exert anti-apoptotic and proliferative effects on human vascular SMC [6,11].

Effects of a deficiency of CX3CL1/CX3CR1 or its blockade in vivo, however, do not allow a discriminatation of local from systemic effects. In this regard, murine aortic transplant models have attracted great attention as these allow studying specific vascular responses caused by the graft itself separate from systemic factors related to the recipient (atherogenic) environment [17–19].

In this study, we focused on the function of CX3CR1 in the atherosclerotic response within an aortic segment graft orthotopically transplanted in mice. This allowed us to investigate the role of vascular CX3CR1 versus systemic CX3CR1 to gain further insight into the details of how this chemokine receptor controls atherosclerotic plaque formation.

Methods

Aortic transplantation

Apoe-/- mice (C57BL/6 background) were crossed with Cx3cr1-/- [20] mice to generate Cx3cr1+/+ Apoe-/- and Cx3cr1-/- Apoe-/- mice. 8–12 week old male mice were housed under standardized conditions in the Animal Facility of the University Hospital Aachen (Germany). The operating procedure was in accordance with European legislation and approved by local German authorities. Infrarenal abdominal Apoe-/- aorta segments were transplanted into Apoe-/- mice (n = 4), Cx3cr1-/- Apoe-/- aorta segments into Apoe-/- mice (n = 5), and Apoe-/- aorta segements were transplanted into Cx3cr1-/-Apoe-/- mice (n = 5). After transplantation, mice were placed on atherogenic diet (21% fat, 0.15% cholesterol, Altromin) for four weeks.

The abdominal aortic transplantation was performed as described previously using the sleeve technique [17,21]. Briefly, mice were anesthetized using a mixture of 1.5 vol. % isoflurane and 100% oxygen through a face mask. The segment of aorta between the renal arteries and its bifurcation was separated from the vena cava. The infrarenal aorta of the recipient was dissected and mobilized between the renal arteries proximally and the bifurcation distally. All the small branches of this segment were secured. The proximal and distal portions of the aorta were clamped by 6/0 single silk suture (Silk, Deknatel, Research Triangle Park NC, USA). The graft was placed in the orthotopic position and the anastomosis was performed using the sleeve technique with sutures 11/0 monofilament (Ethilon, Ethicon, Norderstedt, Germany). The mean surgical anastomosis time was 22 minutes (range 13–40 minutes). Donor and recipient mice were of the same age (8–12 weeks).

Immunohistochemistry

For tissue harvesting, animals were anesthetized (with a mixture of 1.5 vol. % isoflurane and 100% oxygen via a face mask) and vessels were flushed with phosphate-buffered saline (PBS) followed by 4% formaldehyde/PBS (pH 7.4) by cardiac puncture. Grafts were gently removed. After overnight fixation in 4% formaldehyde/PBS, specimens were further processed and embedded in paraffin. Serial sections (5 μm) throughout the transplanted aorta distal and proximal of the anastomosis sites were stained by hematoxylin and eosin staining (HE). Immunocytochemistry was performed using antibodies raised against macrophages (Mac2, CL8942AP/Cedarlane), vascular smooth muscle cells (SMA, M0851/Dako) followed by anti-rat FITC (Jackson Immuno- Research, West Grove, USA) and anti-mouse-Cy3, respectively, antigen KI-67 for cellular proliferation (KI-67, M7249/Dako, Jena, Germany) and TUNEL for detecting DNA fragmentation (1215679210/Roche; 11684795910/Roche, Mannheim, Germany). Positively stained cells were counted in higher magnification (40x) and expressed as percent from total DAPI stained nuclei or as absolute numbers per mm2 (S1A and S1B Fig).

Statistics

Data are presented as mean ± SEM. The significance of changes between experimental groups and different time points was determined by one-way ANOVA, with Tukey multiple comparison test. A p-value of <0.05 was considered significant. Statistical analyses were performed with GraphPad Prism 6.03 (Statcon, Witzenhausen, Germany).

Results

Murine orthotopical transplantations of infrarenal aortic segments of Apoe-/- mice into Apoe-/- mice (control, n = 4), of Cx3cr1-/- Apoe-/- aortic segments into Apoe-/- mice (n = 5), as well as Apoe-/- aortic segments into Cx3cr1-/- Apoe-/- mice (n = 5) were performed using the sleeve technique [17,21], and mice were placed on atherogenic diet containing 21% fat and 0.15% cholesterol. Four weeks after transplantation, the aortic segments were harvested for further analysis.

The histological analysis of the transplanted aortic segment revealed a significant reduction in plaque size in Cx3cr1-/- Apoe-/- aortic segments in Apoe-/- recipients, whereas a trend towards reduced plaque burden was observed in Apoe-/- aortic segments transplanted into cx3cr1-/- Apoe-/- mice did not reach statistical significance, compared to control Apoe-/- aortic segments in Apoe-/- mice (Fig 1). The histological analysis of the transplanted aortic segment revealed a significant reduction in plaque size in Cx3cr1-/- Apoe-/- aortic segments in Apoe-/- recipients, whereas a trend towards reduced plaque burden was observed in Apoe-/- aortic segments transplanted into Cx3cr1-/- Apoe-/- mice did not reach statistical significance, compared to control Apoe-/- aortic segments in Apoe-/- mice (Fig 1). No statistical differences in plaque size could be detected between Cx3cr1+/+ Apoe-/- mice with Cx3cr1-/- Apoe-/- aortic segments and Cx3cr1-/- Apoe-/- mice with Cx3cr1+/+ Apoe-/- aortic segments.

[Figure omitted. See PDF.]

Fig 1. Reduced plaque size after transplantation of Cx3cr1-/-Apoe-/- aortas into Apoe-/- mice.

Apoe-/- mice were transplanted with Apoe-/- aortic segments (n = 4, Apoe-/- > Apoe-/-) or Cx3cr1-/-Apoe-/- aortic segments (n = 5, Cx3cr1-/- > Apoe-/-), and Cx3cr1-/-Apoe-/- mice were transplanted with Apoe-/- aortic segments (n = 5, Apoe-/- > Cx3cr1-/-) and placed on a high fat diet for 4 weeks. Atherosclerotic plaques were analysed in H&E stained sections through the transplanted segment. Quantification of plaque area and representative sections (x20) are shown. *p<0.05, Scale bars 100 μm.

https://doi.org/10.1371/journal.pone.0170644.g001

Immunostaining further revealed that this decrease in atherosclerotic plaque size in Cx3cr1-/- Apoe-/- aortic segments was associated with a significant reduction in the number of smooth muscle actin (SMA)+ SMCs in plaques of the aortic segment (Fig 2A, S1C Fig). The presence of SMA+ SMCs mostly in the intima during plaque formation may indicate that SMCs in the media differentiate towards a synthetic phenotype during vessel inflammation and plaque formation [22]. In contrast, lesional Mac2+ macrophage numbers were not significantly altered between groups (Fig 2B, S1D Fig). These findings suggest that CX3CR1 expressed by vessel wall-resident SMCs is required for atherosclerotic plaques growth in transplanted vessels, whereas its expression on circulating cells and macrophages seems to play a subordinate role.

[Figure omitted. See PDF.]

Fig 2. Reduced numbers of SMCs in transplanted Cx3cr1-/-Apoe-/- aortic plaques.

Apoe-/- mice were transplanted with Apoe-/- aortic segments (n = 4, Apoe-/- > Apoe-/-) or Cx3cr1-/-Apoe-/- aortic segments (n = 5, Cx3cr1-/- > Apoe-/-), and Cx3cr1-/-Apoe-/- mice were transplanted with Apoe-/- aortic segments (n = 5, Apoe-/- > cx3cr1-/-) and placed on a high fat diet for 4 weeks. Immunohistochemistry and quantification of (A) SMCs (alpha-Smooth Muscle Actin staining, x20, red) and (B) macrophages (MAC2, x20, green) in plaques of the transplanted aortic segment. Counterstaining with DAPI (blue) is showed in each images in insert. *p<0.05, Scale bars 100 μm.

https://doi.org/10.1371/journal.pone.0170644.g002

Furthermore, we assessed cell proliferation by Ki-67 staining in all plaque cells and apoptosis by TUNEL staining in all plaque cells but could not detect significant differences between groups (S1E and S1F Fig).

Discussion

We here employed a model of orthotopic transplantation of an infrarenal aortic segment into the infrarenal aorta of recicpient mice. Unlike in bone marrow transplantation models, which can be used to dissect the contribution of bone marrow versus non-bone marrow cells (including vessel wall cells but also all resident cells in other organs), this model allows to focus on the particular contribution of local (transferred) cells within the graft. Using this aorta transplantation model to discriminate between effects of circulating versus local vessel wall resident cells, we here are able to show that interference with the CX3CR1-driven signaling pathway in vessel wall cells inhibits atherosclerotic lesion formation.

Previous studies by Combadière et al. and Lesnik et al. demonstrated a significant decrease in atherosclerotic lesions in mice lacking CX3CR1 [23,24], associated with a reduction in macrophage accumulation in plaques [23,24]. Saederup et al. showed that the deletion of CX3CL1 in CCR2-deficient mice reduced the accumulation of macrophages and the development of atherosclerosis [25]. In accordance, Combadière et al. demonstrated that the combined inhibition of CCL2, CX3CR1, and CCR5 in Apoe-/- mice was associated with a marked and additive reduction in atherosclerosis [26]. The site-specific action of CX3CR1 was not addressed in these studies. However, also bone marrow deficiency of CX3CR1 reduced atherosclerotic lesion formation in chimeric Apoe-/- mice, and the CX3CL1/CX3CR1 signaling pathway was uncovered to exert pro-survival signals in macrophages, whose absence leads to the increased death of monocytes/foam cells during plaque growth [15]. In contrast to these findings, we did not observe significant alterations in plaque size or lesional macrophage accumulation in Cx3cr1-/- Apoe-/- mice transplanted with Apoe-/- mice that entail a deficiency in CX3CR1 in circulating leukocytes. This may be due to specificities of the transplantation model that produces plaques that predominantly contain SMCs rather than macrophages in the infrarenal abdominal aorta.

The interaction of SMCs with monocytes induces a significant up-regulation of CX3CR1 gene and protein expression in both cell types [27]. Moreover, CX3CL1 gene and protein expression increases in the murine aorta in high-fat vs normal diet fed Apoe-/- mice [28]. Notably, CX3CL1 has been demonstrated to exert anti-apoptotic and proliferative effects on vascular cells, mediated via EGFR, with antagonists of CX3CR1 abrogating the proliferative effects of CX3CL1 in SMCs [6]. Deficiency of CX3CR1 may similarly have curtailed CX3CL1-mediated SMC proliferation, in turn inhibiting intimal hyperplasia. However, we cannot rule out the involvement of other vessel wall cells, given that we did not observe changes in SMC or proliferating cells relative to the plaque area. For instance, resident myeloid cells that accumulate CX3R1-dependently in the vessel wall [29] may have contributed to the phenotype observed.

Clinically, stability of an atherosclerotic plaque is an important characteristic [30]. Unstable atherosclerotic plaques are characterized by high numbers of macrophages and decreased SMC and collagen content. These plaques are more likely to undergo rupture and cause vessel thrombosis when compared to SMC and collagen-rich stable plaques [30]. Our findings that a decrease in atherosclerotic plaque size in Cx3cr1-/- Apoe-/- aortic segments was associated lower numbers of SMCs may indicate that inhibition of CX3CR1 may also have unfavorable effects on plaque stability. On the other hand, confining SMC proliferation is major challenge in vascular remodeling after percutanous transluminal coronary angioplasty and stent-implantation [31]. In this regard, targeting CX3CR1 may be a potent therapeutic target limiting monocyte accumulation [15,23,24] and SMC proliferation.

An increased expression of CX3CL1 and CX3CR1 has been found in coronary arteries from patients after heart transplantation, and several studies have suggested a role of CX3CR1 in allograft rejection and dysfunction [13,32–34]. For instance, Robinson et al. observed a prolonged in vivo survival of heterotopic murine cardiac allograft transplants in a major histocompatibility complex-mismatch model, when treated with CX3CR1-antibodies [13]. In our study, however, both donors and recipients were of the C57BL/6 background, excluding the possibility that (CX3CR1-dependent) graft versus host responses may have affected atherosclerotic lesion development in our transplant model.

A clear limitation of our study are the low n-numbers that may have precluded reaching more definite statistical conclusions. In particular, the trend of reduced plaque burden in Apoe-/- aortic segments transplanted into Cx3cr1-/- Apoe-/- mice compared to control Apoe-/- aortic segments in Apoe-/- mice may have substantiated when group sized were lager. Similarly, the cellular plaque characterization yielded values with a wide distribution, so that significant differences between groups may have been missed. Moreover, an additional group of mice with Cx3cr1-/- donors and Cx3cr1-/- recipients is missing to evaluate the complete absence of Cx3cr1 and possible additive effects in our model. Taken together we here unveil an important function of CX3CR1 in resident vessel wall cells to promote atherosclerotic lesion growth in the transplanted abdominal aorta in Apoe-/- mice. Targeting CX3CL1/CX3CR1 may thus be viable therapeutic option in vascular transplantation procedures.

Supporting information

[Figure omitted. See PDF.]

S1 Fig. Assesment of cell content by immunofluorescence.

(A) The positive stained sections for smooth muscle actin (SMA in red) was overlay with DAPI and the nuclei inside the stained area were counted (red arrow heads). Scale bar 50 μm. (B) Similar, nuclei inside the Mac2-stained area (green) are counted (green arrow heads). Immunohistochemistry and quantification of (C) SMCs and (D) macrophages in plaques of the transplanted aortic segment and expressed as cells/mm2. (E) No change is detected after staining with Ki-67 for proliferation and (F) TUNEL for apoptosis.

https://doi.org/10.1371/journal.pone.0170644.s001

(TIF)

S1 Table. The original raw data table.

The original raw data table (in a Excel spreadsheet) that were used to generate our bar graphs.

https://doi.org/10.1371/journal.pone.0170644.s002

(XLSX)

Acknowledgments

We would like to thank Roya Soltan, Melanie Garbe, Stephanie Elbin, and Yuan Kong for their excellent technical assistance.

Author Contributions

1. Conceptualization: ZR TK CW AZ EL.

2. Data curation: ZR AZ EL.

3. Formal analysis: ZR AZ EL.

4. Funding acquisition: ZR TK CW AZ EL.

5. Investigation: ZR TK CW AZ EL.

6. Methodology: ZR TK CW AZ EL.

7. Project administration: ZR TK HS JJ CW AZ EL.

8. Resources: TK HS JJ CW AZ EL.

9. Supervision: TK HS JJ CW AZ EL.

10. Validation: ZR TK MS HS JJ CW AZ EL.

11. Visualization: ZR CW AZ EL.

12. Writing – original draft: ZR TK MS HS JJ CW AZ EL.

13. Writing – review & editing: ZR TK MS HS JJ CW AZ EL.

Citation: Rowinska Z, Koeppel TA, Sanati M, Schelzig H, Jankowski J, Weber C, et al. (2017) Role of the CX3C chemokine receptor CX3CR1 in the pathogenesis of atherosclerosis after aortic transplantation. PLoS ONE 12(2): e0170644. https://doi.org/10.1371/journal.pone.0170644

References

1. Charo IF, Ransohoff RM. The many roles of chemokines and chemokine receptors in inflammation. N Engl J Med. 2006; 354: 610–621. pmid:16467548

2. Back M, Weber C, Lutgens E. Regulation of atherosclerotic plaque inflammation. J Internal Med. 2015; 278: 462–482. pmid:25823439

3. Zernecke A, Shagdarsuren E, Weber C. Chemokines in atherosclerosis: an update. Arterioscler Thromb Vasc Biol. 2008; 28:1897–1908. pmid:18566299

4. Liehn EA, Cabrera-Fuentes HA. Inflammation between defense and disease: impact on tissue repair and chronic sickness. Discoveries. 2015; 3: e42.

5. Fong AM, Robinson LA, Steeber DA, Tedder TF, Yoshie O, Imai T, et al. Fractalkine and CX3CR1 mediate a novel mechanism of leukocyte capture, firm adhesion, and activation under physiologic flow. J Exp Med. 1998; 188: 1413–1419. pmid:9782118

6. White GE, Tan TC, John AE, Whatling C, McPheat WL, Greaves DR. Fractalkine has anti-apoptotic and proliferative effects on human vascular smooth muscle cells via epidermal growth factor receptor signalling. Cardiovasc Res. 2010; 85: 825–835. pmid:19840952

7. Bazan JF, Bacon KB, Hardiman G, Wang W, Soo K, Rossi D, et al. A new class of membrane-bound chemokine with a CX3C motif. Nature. 1997; 385: 640–644. pmid:9024663

8. Ludwig A, Berkhout T, Moores K, Groot P, Chapman G. Fractalkine is expressed by smooth muscle cells in response to IFN-gamma and TNF-alpha and is modulated by metalloproteinase activity. J Immunol. 2002; 168: 604–612. pmid:11777952

9. Greaves DR, Häkkinen T, Lucas AD, Liddiard K, Jones E, Quinn CM, et al. Linked chromosome 16q13 chemokines, macrophage-derived chemokine, fractalkine, and thymus- and activation-regulated chemokine, are expressed in human atherosclerotic lesions. Arterioscler Thromb Vasc Biol. 2001; 21: 923–929. pmid:11397698

10. Postea O, Vasina EM, Cauwenberghs S, Projahn D, Liehn EA, Lievens D, et al. Contribution of platelet CX(3)CR1 to platelet-monocyte complex formation and vascular recruitment during hyperlipidemia. Arterioscler Thromb Vasc Biol. 2012; 32: 1186–1193. pmid:22383701

11. Lucas AD, Bursill C, Guzik TJ, Sadowski J, Channon KM, Greaves DR. Smooth muscle cells in human atherosclerotic plaques express the fractalkine receptor CX3CR1 and undergo chemotaxis to the CX3C chemokine fractalkine (CX3CL1). Circulation. 2003; 108: 2498–2504. pmid:14581400

12. Ruth JH, Volin MV, Haines GK, Woodruff DC, Katschke KJ Jr, Woods JM, et al. Fractalkine, a novel chemokine in rheumatoid arthritis and in rat adjuvant-induced arthritis. Arthritis Rheum. 2001; 44: 1568–1581. pmid:11465708

13. Robinson LA, Nataraj C, Thomas DW, Howell DN, Griffiths R, Bautch V, et al. A role for fractalkine and its receptor (CX3CR1) in cardiac allograft rejection. J Immunol. 2000; 165: 6067–6072. pmid:11086038

14. Apostolakis S, Spandidos D. Chemokines and atherosclerosis: focus on the CX3CL1/CX3CR1 pathway. Acta Pharmacol Sin. 2013; 34: 1251–1256. pmid:23974513

15. Landsman L, Bar-On L, Zernecke A, Kim KW, Krauthgamer R, Shagdarsuren E, et al. CX3CR1 is required for monocyte homeostasis and atherogenesis by promoting cell survival. Blood. 2009; 113: 963–972. pmid:18971423

16. Poupel L, Boissonnas A, Hermand P, Dorgham K, Guyon E, Auvynet C, et al. Pharmacological inhibition of the chemokine receptor, CX3CR1, reduces atherosclerosis in mice. Arterioscler Thromb Vasc Biol. 2013; 33: 2297–2305. pmid:23887641

17. Dambrin C, Calise D, Pieraggi MT, Thiers JC, Thomsen M. Orthotopic aortic transplantation in mice: a new model of allograft arteriosclerosis. J Heart Lung Transplant. 1999; 18: 946–951. pmid:10561104

18. Daugherty A. Mouse models of atherosclerosis. Am J Med Sci. 2002; 323: 3–10. pmid:11814139

19. Xu Q. Mouse models of arteriosclerosis: from arterial injuries to vascular grafts. Am J Pathol. 2004; 165: 1–10. pmid:15215157

20. Jung S, Aliberti J, Graemmel P, Sunshine MJ, Kreutzberg GW, Sher A, et al. Analysis of fractalkine receptor CX(3)CR1 function by targeted deletion and green fluorescent protein reporter gene insertion. Mol Cell Biol. 2000; 20: 4106–4114. pmid:10805752

21. Rowinska Z, Zander S, Zernecke A, Jacobs M, Langer S, Weber C, et al. Non- invasive in vivo analysis of a murine aortic graft using high resolution ultrasound microimaging. Eur J Radiol. 2012; 81: 244–249. pmid:21334152

22. Swier VJ, Tang L, Krueger KD, Radwan MM, Del Core MG, Agrawal DK. Coronary Injury Score Correlates with Proliferating Cells and Alpha-Smooth Muscle Actin Expression in Stented Porcine Coronary Arteries. PlosOne, 2015; 10(9): e0138539.

23. Combadière C, Potteaux S, Gao JL, Esposito B, Casanova S, Lee EJ, et al. Decreased atherosclerotic lesion formation in CX3CR1/apolipoprotein E double knockout mice. Circulation. 2003; 107: 1009–1016. pmid:12600915

24. Lesnik P, Haskell CA, Charo IF. Decreased atherosclerosis in CX3CR1-/- mice reveals a role for fractalkine in atherogenesis. J Clin Invest. 2003; 111: 333–340. pmid:12569158

25. Saederup N, Chan L, Lira SA, Charo IF. Fractalkine deficiency markedly reduces macrophage accumulation and atherosclerotic lesion formation in CCR2-/- mice: evidence for independent chemokine functions in atherogenesis. Circulation. 2008; 117: 1642–1648. pmid:18165355

26. Combadière C, Potteaux S, Rodero M, Simon T, Pezard A, Esposito B, et al. Combined inhibition of CCL2, CX3CR1, and CCR5 abrogates Ly6C(hi) and Ly6C(lo) monocytosis and almost abolishes atherosclerosis in hypercholesterolemic mice. Circulation. 2008; 117: 1649–1657. pmid:18347211

27. Butoi ED, Gan AM, Manduteanu I, Stan D, Calin M, Pirvulescu M, et al. Cross talk between smooth muscle cells and monocytes/activated monocytes via CX3CL1/CX3CR1 axis augments expression of pro-atherogenic molecules. Biochim Bioph Acta. 2011; 1813: 2026–2035.

28. Liu H, Jiang D, Zhang S, Ou B. Aspirin inhibits fractalkine expression in atherosclerotic plaques and reduces atherosclerosis in ApoE gene knockout mice. Cardiovasc Drugs Ther. 2010; 24: 17–24. pmid:19997773

29. Liu P, Yu YR, Spencer JA, Johnson AE, Vallanat CT, Fong AM, et al. CX3CR1 deficiency impairs dendritic cell accumulation in arterial intima and reduces atherosclerotic burden. Arterioscler Thromb Vasc Biol. 2008; 28: 243–250. pmid:18079406

30. Virmani R, Kolodgie FD, Burke AP, Farb A, Schwartz SM. Lessons from sudden coronary death: a comprehensive morphological classification scheme for atherosclerotic lesions. Arterioscler Thromb Vasc Biol. 2000; 20: 1262–1275. pmid:10807742

31. Lenzen MJ, Boersma E, Bertrand ME, Maier W, Moris C, Piscione F, et al. Management and outcome of patients with established coronary artery disease: the Euro Heart Survey on coronary revascularization. Eur Heart J. 2005; 26: 1169–1179. pmid:15802360

32. Hoffmann U, Bergler T, Segerer S, Rümmele P, Krüger B, Banas MC, et al. Impact of chemokine receptor CX3CR1 in human renal allograft rejection. Transpl Immunol. 2010; 23: 204–208. pmid:20600902

33. Cao G, Lu Y, Gao R, Xin Y, Teng D, Wang J, et al. Expression of fractalkine, CX3CR1, and vascular endothelial growth factor in human chronic renal allograft rejection. Transplant Proc. 2006; 38: 1998–2000. pmid:16979977

34. Hu H, Aizenstein BD, Puchalski A, Burmania JA, Hamawy MM, Knechtle SJ. Elevation of CXCR3-binding chemokines in urine indicates acute renal-allograft dysfunction. Am J Transplant. 2004; 4: 432–437. pmid:14961998

Word count: 3801

Show less

© 2017 Rowinska et al. This is an open access article distributed under the terms of the Creative Commons Attribution License: http://creativecommons.org/licenses/by/4.0/ (the “License”), which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited. Notwithstanding the ProQuest Terms and Conditions, you may use this content in accordance with the terms of the License.

Abstract

Background

The CX3C chemokine receptor CX3CR1 is expressed on monocytes as well as tissue resident cells, such as smooth muscle cells (SMCs). Its role in atherosclerotic tissue remodeling of the aorta after transplantation has not been investigated.

Methods

We here have orthotopically transplanted infrarenal Cx3cr1-/-Apoe-/- and Cx3cr1+/+Apoe-/- aortic segments into Apoe-/-mice, as well as Apoe-/- aortic segments into Cx3cr1-/-Apoe-/- mice. The intimal plaque size and cellular plaque composition of the transplanted aortic segment were analyzed after four weeks of atherogenic diet.

Results

Transplantation of Cx3cr-/-Apoe-/- aortic segments into Apoe-/- mice resulted in reduced atherosclerotic plaque formation compared to plaque size in Apoe-/- or Cx3cr1-/-Apoe-/- mice after transplantation of Apoe-/- aortas. This reduction in lesion formation was associated with reduced numbers of lesional SMCs but not macrophages within the transplanted Cx3cr-/- Apoe-/- aortic segment. No differences in frequencies of proliferating and apoptotic cells could be observed.

Conclusion

These results indicate that CX3CR1 on resident vessel wall cells plays a key role in atherosclerotic plaque formation in transplanted aortic grafts. Targeting of vascular CX3CL1/CX3CR1 may therefore be explored as a therapeutic option in vascular transplantation procedures.

Details

Title
Role of the CX3C chemokine receptor CX3CR1 in the pathogenesis of atherosclerosis after aortic transplantation
Author
Rowinska, Zuzanna; Koeppel, Thomas A; Sanati, Maryam; Schelzig, Hubert; Jankowski, Joachim; Weber, Christian; Zernecke, Alma; Liehn, Elisa A
First page
e0170644
Section
Research Article
Publication year
2017
Publication date
Feb 2017
Publisher
Public Library of Science
e-ISSN
19326203
Source type
Scholarly Journal
Language of publication
English
DOI
https://doi.org/10.1371/journal.pone.0170644
ProQuest document ID
1871802876
Copyright
© 2017 Rowinska et al. This is an open access article distributed under the terms of the Creative Commons Attribution License: http://creativecommons.org/licenses/by/4.0/ (the “License”), which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited. Notwithstanding the ProQuest Terms and Conditions, you may use this content in accordance with the terms of the License.