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Continuous wound infusion with chloroprocaine in a pig model of surgical lesion: drug absorption and effects on inflammatory response

Authors Allegri M , Bugada D , De Gregori M, Avanzini MA, De Silvestri A , Petroni A, Sala A , Filisetti C , Icaro Cornaglia A , Cobianchi L 

Received 18 April 2017

Accepted for publication 1 August 2017

Published 31 October 2017 Volume 2017:10 Pages 2515—2524

DOI https://doi.org/10.2147/JPR.S139856

Checked for plagiarism Yes

Review by Single anonymous peer review

Peer reviewer comments 4

Editor who approved publication: Dr Katherine Hanlon



Massimo Allegri,1,2 Dario Bugada,1–3 Manuela De Gregori,2,4 Maria A Avanzini,5 Annalisa De Silvestri,6 Anna Petroni,7 Angelo Sala,7,8 Claudia Filisetti,9–11 Antonia Icaro Cornaglia,12 Lorenzo Cobianchi13,14

1Department of Medicine and Surgery, University of Parma, Parma 2SIMPAR Group (Study in Multidisciplinary PAin Research), 3Department of Anaesthesia and ICU, ASST Papa Giovanni XXIII, Bergamo, 4Pain Therapy Service, Fondazione IRCCS Policlinico San Matteo, 5Laboratory of Transplant Immunology/Cell Factory, IRCCS Foundation Policlinico San Matteo, 6Clinical epidemiology and Biometrics Unit, Fondazione IRCCS Policlinico San Matteo, Pavia, 7Department of Pharmacological and Biomolecular Sciences, University of Milan, Milan, 8I.B.I.M., C.N.R., Palermo, 9PhD School, University of Pavia, 10Department of Pediatric Surgery, Fondazione IRCCS Policlinico San Matteo, Pavia, 11Department of Pediatric Surgery, “V. Buzzi” Children’s Hospital, Milan, 12Department of Public Health, Experimental and Forensic Medicine, University of Pavia, 13Department of Surgical, Clinical, Paediatric and Diagnostic Science, University of Pavia, 14General Surgery 1, IRCCS Fondazione Policlinico San Matteo, Pavia, Italy

Abstract: Continuous wound infusion (CWI) may protect from inflammation, hyperalgesia and persistent pain. Current local anesthetics display suboptimal pharmacokinetic profile during CWI; chloroprocaine (CP) has ideal characteristics, but has never been tested for CWI. We performed an animal study to investigate the pharmacokinetic profile and anti-inflammatory effect of CP during CWI. A total of 14 piglets received an infusion catheter after pararectal laparotomy and were randomly allocated to one of three groups: 5 mL/h infusion of saline (group A), CP 1.5% (group B) and CP 0.5% (group C). Blood sampling was performed to assess absorption and systemic inflammation at 0, 3, 6, 12, 24, 48, 72, 96, 102 and 108 hours. The wound and contralateral healthy abdominal wall were sampled for histological analyses. Absorption of CP from the site of infusion, evaluated as the plasmatic concentrations of CP and its metabolite, 4-amino-2-chlorobenzoic acid (CABA), showed a peak during the first 6 hours, but both CP and its metabolite rapidly disappeared after stopping CP infusion. Local inflammation was reduced in groups B and C (CP-treated p < 0.001), in a CP dose-dependent fashion. While CP inhibited in a dose-dependent manner pig mononuclear cells (MNCs) in vitro proliferation to a polyclonal activator, no effect on systemic cytokines’ concentrations or on ex vivo monocytes’ responsiveness was observed, suggesting the lack of systemic effects, in line with the very short half-life of CP in plasma. CP showed a very good profile for use in CWI, with dose-dependent local anti-inflammatory effects, limited absorption and rapid clearance from the bloodstream upon discontinuation. No cytotoxicity or side effects were observed. CP, therefore, may represent an optimal choice for clinical CWI, adaptable to each patient’s need, and protective on wound inflammatory response (and hyperalgesia) after surgery.

Keywords: continuous wound infusion, pig model, chloroprocaine, pharmacokinetics, inflammation, postoperative pain

Introduction

Postoperative analgesia still remains a challenge,1,2 and the importance of targeted treatments has often been stressed.3,4 Pain involves different mechanisms (peripheral nociception, central modulation and primary and secondary hyperalgesia), with nociceptor’s activation being the trigger for all. Inflammation is the major background factor acting both peripherally and centrally on neural structures, leading to hyperalgesia and probably acting as a main factor toward the development of persistent pain after surgery.5,6

Since the choice of the analgesic strategy should be targeted on pain pathophysiology,7 a rational approach to postoperative analgesia is to block the origin of pain cascade (namely peripheral nociception) and to prevent all pain-related events. Thus, further to subjective pain relief, an effective, prolonged8 nociceptive block should reduce inflammatory response9 and central sensitization.10,11

Continuous wound infusion (CWI) with local anesthetics (LAs) has been documented as an effective technique for postoperative pain relief in several studies12 and comparable to epidural analgesia.13 LAs display local/systemic anti-inflammatory properties, even at low concentrations.14 LAs reduce polymorphonuclear granulocytes’ (PMNs) adhesion in the surgical site and block leukotriene B4, a powerful chemotactic mediator. Lidocaine and ropivacaine reduce TNFα-induced upregulation of integrins (CD11b–CD18) essential for endothelial adhesion and diapedesis into the injured tissue; lidocaine and tetracaine cause loss of PMNs’ round shape necessary for adhesion. The global effect is the reduction of PMNs’ accumulation in the surgical wound, together with the release of local inflammatory chemokines.14

Currently, drugs used for CWI are long-lasting LAs, such as ropivacaine, bupivacaine, and levobupivacaine. Such drugs are considered safe at clinical doses, and the kinetic profile and blood levels have already been investigated during epidural infusions.15

However, both from a clinical and a pharmacokinetic perspective, an ultra short-acting LA may be more appropriate for CWI, as it could be better modulated according to specific patients’ needs with “on/off” profile.

Chloroprocaine (CP) has fast onset (6–10 minutes) and short action (around 90 minutes),16 with a cholinesterase-based plasmatic metabolism. Early cases of toxicity after spinal anesthesia17 were documented, but were related to the sodium bisulfite antioxidant and to the solution’s low pH.18 Nowadays, antioxidant-free, safer preparations are available, and interest has grown again because of CP’s ideal profile for CWI.

There is no study, to our knowledge, investigating CP during intrawound continuous infusion in an animal model; moreover, there are few data elucidating the effect on local and systemic inflammation of a continuous subfascial wound infusion of LAs and in particular for CP.

As recently underlined by Gigliuto et al,19 a large animal model could be more appropriate than others to produce reliable translational results. We therefore evaluated the absorption associated with a continuous CP intrawound (subfascial) infusion in pig. We also investigated if CP at two different dosages may influence local and systemic inflammatory responses after surgical lesion both in vivo and ex vivo.

Materials and methods

All animal procedures were performed according to the protocol approved by Institutional Animal Care and Use Committee (IACUC) – University of Pavia. All animal care and experimental procedures followed local, national and European Union guidelines for the animals’ use (Directive 2010/63/EU – revising Directive 86/609/EEC on the protection of animals used for scientific purposes).

Animals and surgical procedures

Piglets (20–30 kg) underwent pararectal laparotomy, extended for 10 cm. The parietal peritoneal membrane was then closed with a continuous absorbable synthetic suture. An intrawound, multiholed catheter (PAINFusor® – Plan-1-Health, Udine, Italy) was placed between peritoneum and deep muscular fascia along the length of the wound and tunneled subcutaneously. Muscle layers and skin were finally closed with a continuous absorbable synthetic suture.

Surgical procedure was performed under general balanced anesthesia, including mechanical ventilation via orotracheal intubation and mioresolution.20,21 A central venous catheter was placed in the right external jugular vein with open surgical technique and was used for drug infusion and for blood sampling. At the end of surgical procedures, piglets were set in the metabolic cage and were supplied with water and standard bran. Intravenous antibiotic (cefazolin 1 g) and omeprazole 40 mg were administered during follow-up to prevent wound infections and stress-induced gastric ulcerations. Analgesia was performed in all animals by intramuscular injection of tramadol 50 mg during the perioperative period, with no additional analgesics, according to our animal protocols for surgical trials.

Animals were randomly allocated to 3 groups with a 5 mL/h continuous infusion through elastomeric pump for 72 hours: saline (group A), CP 1.5% (group B) or CP 0.5% (group C). The randomization was based on a computer-generated list.

Sample collection

During the follow-up period, peripheral blood was collected for the determination of CP and its metabolite, as well as of the effects on systemic inflammation, at 0, 3, 6, 12, 24, 48, 72, 96, 102 and 108 hours from incision. Plasma was obtained by centrifugation at 3000 rpm for 15 minutes and stored at –20°C until analysis. Mononuclear cells (MNCs), for in vitro and ex vivo experiments, were obtained by gradient density on cell separation media (Cedarlane, Burlington, USA) at 2500 rpm for 20 minutes. The catheter was removed after 96 hours of infusion. Piglets were finally sacrificed, according to international guidelines.

Determination of CP and its metabolite in plasma

CP and its metabolite 4-amino-2-chlorobenzoic acid (CABA) were analyzed by liquid chromatography/tandem mass spectrometry using a high performance liquid chromatography (HPLC) Agilent (model 1200) equipped with an autosampler (PAL HTS-xt; PAL System, CTC Analytics, Zwingen, Switzerland) directly interfaced with a triple-quadruple API 4000 (AB Sciex, Framingham, MA, USA), equipped with an electrospray ionization (ESI) source.22,23 CP was provided by Sintetica SrL, (Mendrisio, Switzerland) CABA by Sigma-Aldrich Co. (St Louis, MO, USA) and deuterated PABA (4-aminobenzoic acid), used as internal standard (IS) for chloroprocaine and CABA quantitation, by Santa Cruz Biotechnology Inc., Dallas, TX, USA. Methanol and formic acid were from Sigma-Aldrich, whereas HPLC grade water was obtained using a Milli Q water purification system. Chromatographic separation was carried out using a Synergi 4 micro-Hydro-RP 80 A, 150 × 2 mm × 4 µm column (Phenomenex, Torrance, CA, USA) at a flow rate of 200 µL/min. A total of 10 µL of the sample was injected in a linear gradient system from 85% of solvent A (0.1% formic acid in water) to 90% of solvent B (0.1% formic acid in methanol) over 3 minutes. Final conditions were held for 3 minutes before equilibration back at starting conditions.

The triple-quadruple was operated in positive ions mode for multiple reaction monitoring (MRM). The following characteristic fragmentations were used for identification and quantitative analyses: CP from m/z 272 to 198.6 or 153.9, CABA from m/z 172.2 to 128 or 153.9, and d4-PABA from m/z 142.1 to 98.8 or 123.9. The most abundant transition was used for quantitative analysis, while the second transition was used as qualifier for additional identification purposes. A total of 100 µL of plasma samples were added with 20 µL (1 ng/µL) IS and 400 µL of methanol; samples were then put at –20°C overnight. After centrifugation at 13,000 rpm for 10 minutes, 450 µL of the solution were recovered and evaporated using a rotary evaporator. Finally, the samples were resuspended in 100 µL of water/methanol (1:1) and 10 µL was used for liquid chromatography/tandem mass spectrometry analysis. The calibration curves were prepared in drug-free pig plasma, from working solutions of CP and CABA of 1, 3, 10, 30, 100 and 300 ng/mL and processed as the biological samples. Calibration curves were obtained plotting the ratio of the chromatographic area of specific transitions for the compounds of interest over that of specific transition of the internal standard, and the correlation coefficient was always better than 0.99. The limit of quantification (LOQ) was 1 ng/mL of plasma for both compounds.

Data were acquired and processed using Analyst 1.6.1. Concentrations are presented as mean and standard error of the mean of n determinations.

Histopathological analysis

For histological examination, 3 samples of the full-thickness wound and 1 sample of the contralateral healthy abdominal wall were collected from each animal. Each sample was 0.5 cm thick. The samples were fixed in 4% neutral buffered formalin for 48 hours, dehydrated with gradient alcohol series, cleared in xylene and eventually embedded in paraffin. Serial sections (8 μm) were obtained using a Leitz (Wetzlar, Germany) microtome, stained with hematoxylin and eosin (H&E) and examined with a Zeiss (Oberkochen, Germany) Axiophot microscope.

We evaluated the presence of inflammatory cells: neutrophils, eosinophils, lymphocytes, macrophages and mast cells, in pericatheter blank tissues. A total of 15 sections were evaluated for statistical analysis (4 sections per group – corresponding to a different animal of each experimental group plus 1 contralateral healthy sample per group). For each section, at least 8 randomly determined areas of connective tissue were examined at 20× magnification and 100 cells per area were counted. The rate of inflammatory cells was assessed using a semiquantitative scale, with scores ranging from 0 to 4 by 3 independent observers (Table 1). Histological scores are reported as median and 25–75 percentile (interquartile range, IQR).

Table 1 Semiquantitative score used for the assessment of the percentage of the inflammatory infiltrate

Systemic inflammation analysis

Systemic inflammation was evaluated by quantifying pig interleukin-6 (pIL-6), pIL-10, pIL-8, pIL-1β and pig interferon (pIFN)-γ levels in plasma samples at each time point, after incision in all animals, by commercially available quantitative enzyme-linked immunosorbent assay (ELISA) (Quantikine; R&D Systems, Inc., Minneapolis, MN, USA). Detection limits were as follows: 18.8 pg/mL for pIL-6, 31.3 pg/mL for pIL-10, 62.5 pg/mL for pIL-8, 39.1 pg/mL for pIL-1β and 39 pg/mL for pIFN-γ.

In vitro and ex vivo cell proliferation suppression

In order to evaluate in vitro cell proliferation suppression, CP and CABA were added at different concentrations (from 1.25 to 0.02 mg/mL) to resting and phytohemagglutinin (PHA)-activated MNCs obtained before treatment. In detail, 105 MNCs/well were plated in triplicate in flat-bottom microwells (Corning Costar, Euroclone, Milan, Italy), in RPMI 1640 medium (ThermoFisher Scientific, Waltham, MA, USA), 10% fetal calf serum (Euroclone, Celbio), without (resting) or with PHA (activated) (4 g/mL; Boehringer Ingelheim, Mannheim, Germany). After a 3-day incubation at 37°C in a humidified 5% CO2 atmosphere,3 H-thymidine (3HTdR 0.5 mCi/well; Amersham, Buckinghamshire, UK) incorporation was measured during the last 21 hours by standard procedure. Results were expressed as stimulation index (SI = cpm stimulated/cpm unstimulated) and reported as residual proliferation.

Moreover, in order to define if CP in vivo treatment induced a change in cell response capability we evaluated ex vivo, with the same methodology, the effects of CP treatment on the response to PHA of MNCs obtained at different time points (basal, 96 and 108 hours) of pharmacological treatment in groups A (saline), B (CP 1.5%) and C (CP 0.5%).

Cell viability

To test if CP and CABA could affect MNCs viability, after in vitro culture, cells were evaluated by Trypan blue (Sigma, Milan, Italy) exclusion test. Percentage of cell viability is calculated as (number of viable cells/total number of cells [viable + nonviable] × 100).

Statistical analysis

Cytokine concentrations were compared between groups with analysis of variance for repeated measure. An ordinal logistic regression model was fitted using histological score as dependent variable and group as independent variable. To compare all groups, post hoc estimation (between doses or between groups B and C and group A) and Wald tests were also performed. A p-value <0.05 was considered statistically significant.

Quantitative variables are described as mean and SD. Comparisons between groups (A and B, C) and time were performed by means of analysis of variance for repeated measures. The same method was applied to analyze SI at different CP and CABA concentrations. Robust standard errors were considered to take into account the clustered nature of the data. A p-value <0.05 was considered significant. Stata v14.1 (StataCorp LP, College Station, TX, USA) was used for all the analyses.

We did not perform a power analysis since previous literature does not provide data to support any power calculation. The present study is to be considered as a pilot study.

Results

Four animals (25–30 kg, average weight 29.6 kg) were randomly allocated to each group; in group A 2 additional animals were studied as 2 animals were excluded as they developed fever and wound infections. All the other animals in groups B and C completed the follow-up period uneventfully, and they were all treated without any deviation from the protocol.

We did not register any adverse effect or allergic reaction in all the animals used for the study.

Concentrations of CP and its metabolites in plasma

Concentrations of CP were mostly below the quantitation limit, with only 6 blood samples showing the presence of very low concentrations of the intact molecule (1–2.3 ng/mL in animals perfused with CP 0.5%, and 1–20.8 ng/mL in animals perfused with CP 1.5%). CABA concentrations showed a sharp increase immediately after the infusion was started, peaking between 3 and 6 hours from the beginning of the infusion, and returning to basal level (zero) as soon as the continuous infusion was stopped (Figure 1). The peak in CABA concentrations appeared to be proportional to the concentration of CP infused (Figure 1), averaging 177±141 and 543±169 ng/mL in animals perfused with CP 0.5% and 1.5%, respectively.

Figure 1 CABA plasma concentrations after continuous infusion with 0.5% (closed squares) and 1.5% (closed diamond) of chloroprocaine.

Note: CABA was measured by liquid chromatography/tandem mass spectrometry as described in the “Materials and methods” section. Data are expressed as mean and SEM (n = 4).

Abbreviations: CABA, 4-amino-2-chlorobenzoic acid; CP, chloroprocaine; SEM, standard error of the mean; h, hours.

Histopathological analysis

The presence of inflammatory cells was significantly higher in group A than in groups B and C (p < 0.001, in both cases). These results are well summarized by semiquantitative scores (Table 2) that show a dose-dependent reduction of the inflammatory infiltrate within the wound, which is nearly halved with higher CP doses.

Table 2 Trend of the inflammatory infiltrate scores among the different treatments

Abbreviations: CP, chloroprocaine; IQR, interquartile range.

This reduction is even more evident in wound sections, where refined analyses on tissue damage and reaction are possible: pigs in group A (saline) have high amounts of leukocytes and lymphocytes infiltrating wound layers up to connective tissue, and cells surrounding the catheter’s blank display signs of necrosis (Figure 2). Signs of cell damage are less evident in CP-infused pigs, and inflammatory infiltrates are less pronounced and different in nature (less leukocytes); inflammation reaches the connective tissue to a lesser extent, and signs suggestive of tissue regeneration are evident (Figure 3). The reduction in inflammatory infiltrates and signs of tissue regeneration are more evident with higher doses of CP (Figure 4), however no statistically significant difference was observed between groups B and C (Table 2).

Figure 2 Group A (saline) animal.

Notes: (A) Catheter blank (white in the picture) surrounded by connective tissue. A large amount of inflammatory infiltrate is evident, mostly round cells such as lymphocytes and some PMNs. (Inset) Right next to the blank, many cells appear pale as if suffering or necrotic; collagen fibers are contracted. Many red blood cells are present, probably due to the catheter extraction. (B) Inflammation reaches the cutaneous connective tissue, while (C) a great number of leukocytes surround muscular fibers (D) and contralateral healthy skin appears normal.

Abbreviations: CP, chloroprocaine; PMN, polymorphonuclear granulocyte.

Figure 3 Group B (CP 1.5%) animal.

Notes: (A) Connective wall surrounding the blank shows no structural damage in comparison with controls; inflammatory infiltrate appears less evident, just few leukocytes are present, mostly lymphocytes; (inset) fibroblasts look plump and basophilic; collagen bundles are thin with an irregular arrangement and some tiny blood vessels are evident, suggesting tissue repair. (B) Cutaneous tissues contain a slightly higher amount of infiltrate than contralateral healthy skin (D). (C) Muscular fibers are surrounded by few leukocytes.

Abbreviation: CP, chloroprocaine.

Figure 4 Group C (CP 0.5%) animal.

Notes: (A) Connective tissue of the blank wall contains active basophilic fibroblasts, thin collagen bundles and a number of round white blood cells (inset); (B) mild inflammatory infiltrate affects dermal papillae and (C) intramuscular connective. (D) Contralateral healthy skin appears normal.

Abbreviation: CP, chloroprocaine.

Systemic inflammatory analysis

Plasma cytokine quantification at different time points did not reveal any statistical differences between groups B and C versus group A, respectively, for the pro-inflammatory cytokines’ levels (IL-1β, p = 0.8 and 0.4; IL-6, p = 0.7 and 0.9; IL-8, p = 0.6 and 0.6; IFN-γ, p = 0.06 and 0.2) and those of the anti-inflammatory ones (IL-10, p = 0.3 and 0.3) during the entire follow-up period (Figure 5).

Figure 5 Trend of the blood cytokines levels in the three experimental groups.

Notes: Group A, saline; Group B, CP 1.5%; Group C, CP 0.5%.

Abbreviations: CP, chloroprocaine; IL, interleukin; IFN, interferon.

In vitro and ex vivo cell proliferation analyses

The effect of CP and its metabolite on the in vitro proliferation of pig MNCs stimulated with PHA was evaluated at different concentrations in 4 animals using MNCs obtained before any kind of surgical procedure and treatment. The results are shown in Figure 6.

Figure 6 Treatment group in vitro proliferation.

Notes: In vitro cell proliferation suppression by CP (A) and its metabolite (B) at different concentrations, on PHA-activated pig MNCs. Results are expressed as residual proliferation. CP induces significant reduction at concentration of 1.25 mg/mL (*p = 0.012) and of 0.6 mg/mL (**p = 0.052). (C) In vitro PHA-induced proliferation of MNCs obtained from group A, B, C animals at different time points (gray bars = T0, black bars = 96 hours and white bars = 108 hours). Results are expressed as stimulation index. No significant differences are observed between treated and control groups. Group A, saline; Group B, CP 1.5%; Group C, CP 0.5%.

Abbreviations: CP, chloroprocaine; MNCs, mononuclear cells; PHA, phytohemagglutinin.

PHA-stimulated proliferation of MNCs was significantly reduced by the addition of 1.25 and 0.6 mg/mL of CP, with a direct correlation between the concentrations and the degree of inhibition. A decrease in proliferation was also observed for CABA at 1.25 mg/mL, but it was not statistically significant (p = 0.1).

Evaluation of cell viability, by Trypan blue exclusion test, showed that the addition of CP and CABA to in vitro resting and activated pig MNCs did not cause cell death, even at the highest concentration (percentage of viable cells 72% and 79%, respectively), suggesting the lack of cytotoxic activity of CP and its metabolite. Moreover, CP and CABA did not induce in vitro cell proliferation at any concentrations of resting MNCs, indicating no antigenic activity.

In order to assess the effect of CP and CABA we evaluated ex vivo the response to PHA of MNCs isolated from blood collected at different time points (basal, 96 and 108 hours). Results did not show any significant differences between group A versus group B (p = 0.22) and versus group C (p = 0.34) at each time point.

Discussion

So far, long-acting LAs have mainly been used for CWI, despite their suboptimal pharmacokinetic profile and the lack of studies investigating their systemic exposure.

New formulations of CP, an ultrashort acting LA with plasmatic pseudocholinesterase metabolism, theoretically display an ideal pharmacokinetic profile for CWI. In a translational perspective, and responding to the need of testing this molecule in an experimental setting, we investigated the use of CP in a large animal model (pig).

The current investigation confirmed the hypothesis that CWI in our large animal model would result in relatively low amounts of CP being absorbed, and in light of the extremely short half-life of CP in plasma may definitely limit the possibility of systemic effects: indeed during the 96 hours of 5 mL/h continuous administration of both 0.5% and 1.5% CP, the overall amount of CP penetrating the systemic circulation (that is plasma concentrations of CP + its plasmatic metabolite CABA) reached an average Cmax at least 10-fold lower than that observed in obstetric patients receiving epidural CP during cesarian section.24 A dose-related increase in concentrations was observed after the beginning of the CWI and up to 6 hours, suggesting an initial blood vessel-dilating response to CP,25 resulting in a peak of absorption that appeared to progressively decrease over time. We registered no side effects or allergic reaction in any of the enrolled animals. Our study confirms CP as an ideal local anesthetic for CWI, due to its fast catabolism, safety and on/off profile.

The lack of a cholinesterase inhibitor at collection prevents the actual assessment of systemic exposure to intact CP since CP degradation occurs very rapidly in plasma, but reporting the total amount of CP entering the bloodstream (that is CP + CABA) our study reliably describes the overall absorption of CP upon CWI, showing concentrations well below those observed upon epidural administration during either cesarean section or vaginal delivery,24 peaking between 3 and 6 hours and decreasing to undetectable levels after infusion was suspended. Therefore, also taking into account potential differences in esterase activities between the experimental animal used and humans, the systemic exposure to CP appeared very limited, as confirmed by the lack of effects on inflammatory parameters or blood cell activity. Indeed no correlation was detected between treatment and systemic inflammation, as assessed by determination of plasma concentrations of pro-inflammatory cytokines, suggesting that only local inflammation was modulated by the presence of CP. Additionally, local infusion of CP did not affect the ex vivo response of immune cells obtained from treated animals, even if PHA-induced proliferation of MNCs was suppressed by in vitro addition of CP, further supporting the lack of significant circulating concentrations of intact CP as suggested by the relatively low plasmatic concentrations of CABA.

Our data also suggest that the continuous infusion with CP displays local anti-inflammatory effects. These effects were dose-dependent, as we observed a more pronounced reduction of inflammatory response in the group treated with higher concentrations of local anesthetic. Since we did not monitor pain, we cannot determine if the dose-dependent anti-inflammatory effect is associated with either better pain relief, or with a more pronounced reduction of neurogenic inflammation or with specific anti-inflammatory effect of CP. Investigating the pain response would have provided additional support to our studies, but measuring pain in a large animal model can be very challenging, and a well-accepted model is still lacking. Nevertheless, apart from the assessment of the analgesic effect, our study was able to confirm in a large animal model results previously obtained only in small animals,26,27 ie, the ability of nociceptive block to reduce local inflammation. In consideration of the promising results relative to the limited absorption and the anti-inflammatory effect of CP obtained with this study, future trials are warranted to address this topic.

Despite the low sample size (typical of studies in big animal models19), we confirmed the limited absorption and a local anti-inflammatory activity of CWI with CP. Once these results are confirmed in humans, they may show CP to be a good choice for CWI allowing immediate analgesic benefit and fast elimination; patients with liver or kidney diseases may take advantage of rapid plasmatic clearance of CP, preventing accumulation and toxicity. Clinical studies are needed to define the lowest effective dose of CP and investigate its anti-inflammatory effect in a human model.

Conclusion

This pilot study on CP continuous infusion in a large animal model may display future translational value. Once confirmed in humans, our data may show CP to be a first-line choice for CWI, with limited systemic exposure, high compliance to the needs of each patient and potential applications to a broad spectrum of clinical situations. The dose-dependent anti-inflammatory effect may have clinical relevance in pain medicine, showing CP to be an interesting target for future clinical applications and research purposes.

Acknowledgment

The authors would like to thank the following colleagues as strong contributors to this study: Tommaso Dominioni and Andrea Peloso – Department of Surgical, Clinical, Paediatric and Diagnostic Science, University of Pavia, and General Surgery 1, IRCCS Fondazione Policlinico San Matteo, Pavia, Italy; Andrea Fanelli – Department of Anaesthesiology and Intensive Care, Azienda Ospedaliero-Universitaria Policlinico S. Orsola-Malpighi, Bologna, Italy; Daniela Ghisi – Department of Anaesthesia and Postoperative Intensive Care, Istituto Ortopedico Rizzoli, Bologna, Italy; Giovanna Riccipetitoni, Department of Pediatric Surgery, “V. Buzzi” Children’s Hospital, Milan, Italy; Patrizia Risé – Department of Pharmacological and Biomolecular Sciences, University of Milan. The study has been funded by a grant by the Italian Health Ministry (“New nanotechnology and biomedical approaches to improve postoperative pain treatment reducing risks related to opioids” – GR-2010-2318370; Principal Investigator Massimo Allegri, MD) and a grant by Foundation “Banca del Monte di Lombardia” (“La Nanotecnologia applicata al Trattamento del dolore”; Principal Investigator Lorenzo Cobianchi, MD). The authors would like to thank Sintetica® for providing Chloroprocaine for this study.

Disclosure

The authors report no conflicts of interest in this work.

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