Barrier Effect of a New Topical Agent on Damaged Esophageal Mucosa: Experimental Study on an ex vivo Swine Model.

PURPOSE: AL2106 is a new medical device based on a mixture of chondroitin sulphate in a xyloglucan and glycerol solution made to maximize its bioadhesive capability to the esophageal mucosa. The aim of the present study was twofold to evaluate the AL2106 protective effect on the esophageal mucosa when exposed to an acidic solution mimicking gastric reflux and to assess the resilience of this effect to saline washing.
MATERIALS AND METHODS: A porcine ex vivo model was used and the effects of the new medical device were compared to a sodium alginate suspension (SAS) already present on the market which was assumed as reference. Mucosal damage was induced in 19 porcine esophagi by perfusion with an acidic solution added with pepsin, and Evans blue dye (EBD) tissue uptake was used as an indicator of mucosal permeability. The EBD penetration, expressed as EBD µg/g of dry tissue, was assessed in specimens of untreated damaged mucosa and in specimens treated with AL2106 or SAS. The same evaluation was carried out after washing with normal saline.
RESULTS: Both topical agents tested significantly reduced the EBD uptake by more than 60% (AL2106 8.4±4.5, SAS 3.6±2.7 vs control 23.2±13.1, p<0.01). The saline washing did not cause any significant reduction in the protective effect of AL2106 (8.6±5.9), while it significantly reduced that of SAS (5.9±4.3, p<0.05).
CONCLUSION: The new AL2106 medical device showed a good barrier effect against a reflux-like damaging solution and preserved this effect after the mucosal washing test, thus suggesting its possible relevance for the treatment of gastroesophageal reflux disease.

Introduction

Gastroesophageal reflux disease (GERD) is a condition affecting 10–20% of the Western population. It is now well established that the mechanisms underlying symptoms in GERD patients are not only related to esophageal acid exposure, but also to enhanced esophageal sensitivity due to increased mucosal permeability, thus explaining the partial failure of anti-secretory therapy in these patients.1–4

The esophageal mucosa consists of a stratified squamous epithelium which acts as a tight defensive barrier against the injurious components of the gastroesophageal refluxate, and its impairment has been demonstrated not only in patients with mucosal erosions (esophagitis) but also in those with an apparently normal mucosa (NERD), who represent the most common GERD phenotype.5–7

In recent years, several experimental studies aimed at demonstrating the possibility of strengthening the mucosal barrier by means of topical products containing combinations of hyaluronic acid, chondroitin sulfate, alginates and antacids have been carried out on both animal models and humans.7–11

In a previous study, the Authors demonstrated how perfusion with a hyaluronic acid- and chondroitin sulfate-based product (Esoxx®) was able to reduce the permeability of the acid/peptic-damaged esophageal mucosa in a porcine ex vivo model in which the epithelial permeability was assessed using Evans blue dye (EBD) visualization on microscope sections.7

AL2106 is a new formulation for medical device, potentially useful for the topical treatment of GERD symptoms, based on a new mixture of chondroitin sulphate (CS), xyloglucan and glycerol aimed at increasing its bioadherence to the esophageal mucosa.

The aim of the present study was to evaluate, using a porcine ex vivo established model, the potential barrier protective effect on the esophageal mucosa of this new original chemical formulation and its bioadhesive capability by assessing its resilience to washing events.

Materials and Methods

Organ Collection and Preparation

The esophagi were collected from commercially available European breed pigs, weighing approximately 120 kg, at a local slaughterhouse immediately upon slaughter, and transferred within 2 hours in cooled saline to the physiology labs of the Department of Veterinary Medical Sciences of the University of Bologna. The organs were obtained at the slaughterhouse from carcasses earmarked for human consumption, thus replacing the slaughter of animals for tissue sampling in accordance with the 3Rs (Reduction, Replacement and Refinement). Therefore, it ethical approval was not needed as no animal had been sacrificed for experimental purposes.

Only organs without visible lesions were used for the experimental purposes (n=19). Upon arrival, each esophagus was thoroughly rinsed with tap water (inside and outside), and the cranial and caudal sphincters were ablated. The adventitial and the muscular layers were removed, maintaining only the submucosal and mucosal layers; the organs were then pinned upright (cranial end at the top and caudal end at the bottom) on an polystyrene support and placed in a thermostatic hood (Climatic Hood 810; ASAL s.r.l, Cernusco sul Naviglio, Italy) set at 37°C with an inclination of approximately 45 degrees as previously described7 (Figure 1).

Figure 1

Porcine esophagus ex vivo model. An esophagus ablated of its adventitial and muscular layers (A) An esophagus ablated of the lower sphincters, pinned to the support, attached to a perfusion pump, and placed in the thermostatic hood (B).

Once positioned, the cranial opening of the esophagus was secured by means of a surgical knot to an extension tube connected to a 50 mL syringe attached to a perfusion pump. At the beginning of the experiment in order to obtain regular and uniform perfusion, the caudal end was closed by means of a surgical knot, and the esophagus was filled with 40 mL of the damaging solution for 5 minutes. At this point, the caudal surgical knot was removed and perfusion with the damaging solution started. The perfusion rate was set to 60 mL/h and lasted 60 minutes. Due to an inclination of approximately 45 degrees, the damaging solution was also slowly cleared from the aperistaltic esophagi.

Damaging Solution

Mucosal damage was achieved with an acidic-peptic solution. In particular, the damaging solution was prepared by adding porcine pepsin (2000 U/mL, Sigma-Aldrich, St. Louis, MO, USA) to normal saline acidified to pH 2 with HCl 0.1 N and warmed to 37°C. In the Authors’ previous study, it was found that this solution was able to induce microscopic mucosal damage on all the esophagi perfused.7

Design of the Study

At the end of the perfusion with the damaging solution, the esophagi were longitudinally sectioned, and the exposed inner mucosa was washed for 5 minutes in normal saline. At this point, six tissue fragments (~1cm x 1cm) were obtained from the middle portion of each organ and were used for the EBD quantitative analysis. The quantitative data were corroborated by a qualitative evaluation of tissue fragments using a microscope to indicate the depth of the EB penetration. The esophageal fragments underwent different treatments according to the strategy schematized in Figure 2. Briefly:

Figure 2

Design of the study. Mucosal sampling and sequence of treatments after perfusion with the damaging solution. Six samples were taken from each esophagus. One served as epifluorescence control (CTR), one was stained with Evans blue dye (EBD) immediately while the others were treated with topical agents and stained with EBD, preceded or not by washing with saline.

One untreated fragment was used as a control for the epifluorescence evaluation.

One fragment was exposed to the EBD solution (10 mg/mL in normal saline solution; Sigma-Aldrich, St. Louis, MO, USA) for 10 minutes.

Two fragments were treated with each of the two products tested for 10 minutes, and were then exposed to the EBD solution for 10 minutes.

The products were each in stick packs of 10 mL:

AL2106: a new mixture of chondroitin sulphate in a bioadhesive solution of xyloglucan and glycerol polymer.

SAS: suspension of sodium alginate and potassium bicarbonate.

4. Two fragments were treated with each of the two products tested for 10 minutes and were then washed for 30 seconds with normal saline before exposure to the EBD solution for 10 minutes.

At the end of the above-mentioned procedures, all the fragments were washed twice in normal saline solution; the first wash was very rapid consisting of two dips in 100 mL of saline solution while the second one was 5 minutes long in 50 mL of saline. The fragments were then trimmed and divided into three approximately equal samples: one earmarked for epifluorescence evaluation and two as technical duplicates for EBD quantification.

Mucosal Permeability Assessment

The presence of the EBD inside the tissue was used as an indicator of increased permeability caused by peptic/acid perfusion since intact mucosa does not absorb the dye. To evaluate the quantity of EBD penetrated, a method of EBD extraction and spectrophotometric quantification was used.

In addition, a qualitative evaluation with an epifluorescence microscope was carried out.

Extraction and Quantification of the EBD

All the samples were dried at 37°C in a thermostatic hood for 30 minutes and were then immediately weighed, placed in a 15 mL conic tube with 3 mL of formamide (Sigma-Aldrich, St. Louis, MO, USA) and incubated for 48 hours at 50°C. The quantity of EBD extracted from the tissue was evaluated using spectrophotometric measurements (Gene Quant 1300; GE Healthcare, UK) at the absorption maximum for Evans Blue (620 nm). Micrograms of EBD per g of tissue were quantified using a standard curve (0.025–25μg/mL EBD in formamide) and each of the sample weights. The data of the two technical replicates were averaged.

Evaluation of EBD Penetration Using Epifluorescence Microscopy

To evaluate the EBD penetration using epifluorescence microscopy, the esophagus fragments were fixed in 4% buffered formic aldehyde (pH 7.4) overnight at 4°C. The next day, after a short wash in phosphate buffered saline (PBS), the fragments were transferred into a 25% sucrose PBS solution at + 4°C to give protection against subsequent cryopreservation. Upon complete precipitation, the samples were embedded in optimal cutting temperature (OCT) compound (Sakura Finetek, USA) and stored at −80°C. Ten μm thick esophageal mucosal/submucosal serial sections were cut at a Leica CM1950 cryostat (Leica, Wetzlar, Germany) and were placed on microscope slides. The samples were observed using an Eclipse E600 epifluorescence microscope (Nikon Europe BV, Badhoevedorp, The Netherlands) equipped with a Nikon DXM 1200 digital camera.

Statistical Analysis

All the quantitative EBD tissue uptake data were expressed as mean ± standard deviation (SD); single comparisons were carried out using the paired and unpaired Student’s t-test (parametric data) where appropriate. Significance was set at a value of p < 0.05.

Results

Assessment of Mucosal Permeability

In the present study, 19 esophagi were damaged using an acidic/peptic solution, and 6 mucosal fragments were collected from each of them. According to the design of the study (Figure 2), of the 114 samples, 95 were stained with the EBD solution, and the presence of the dye inside the fragment was used as a measure of the mucosal permeability. The EBD absorption values were expressed as EBD µg/g of tissue.

The first analysis was carried out by comparing the EBD absorbed values in the two sample subgroups. As expected, the absorption values of the mucosal samples treated were significantly lower than those of the damaged but untreated mucosal fragments (Figure 3). A statistically significant reduction (p<0.01) in EBD penetration was observed after treatment with both AL2106 (8.4±4.5 µg/g) and SAS (3.6±2.7 µg/g) when compared with the control fragments (23.2±13.1 µg/g), confirming their protective properties. Assessment of the barrier effect after washing with saline showed that the effect persisted without variation for AL2016 (8.6±5.9 µg/g) while it showed a significant barrier effect reduction for SAS (5.9±4.3 µg/g).

Figure 3

The quantity of Evans blue dye (EBD) (µg/g) in the damaged mucosa treated with AL2106 and SAS. The data, expressed as a column chart, represent the mean ± standard deviation (SD) (vertical bars). EBD values in µg/g of dry tissue; Paired and unpaired Student’s t-test (parametric data).

Since the absorbance values observed in the untreated samples were rather variable (range 7.6–52.7 µg/g), potentially due to the variability depending on different animals and “on field” sampling conditions, the difference between each treatment and the corresponding control value obtained from the same esophagus was calculated, assuming that the fragments obtained from the same esophagus had the same behavior. Figure 4 shows the difference observed after the treatments with respect to their control values; higher values indicated a greater reduction in EBD absorption due to an improvement in the mucosal barrier. The results in the unwashed samples showed a reduction of 14.8±14.9 µg/g for AL2106 and of 19.6±12.3 µg/g for SAS. As observed for the absolute values, the saline washing did not modify the effect of AL2106 (14.6±14.3 µg/g) but it reduced that of SAS. (17.3±12.4 µg/g, p<0.05).

Figure 4

The quantity of Evans blue dye (EBD) (µg/g) in the damaged mucosa treated with AL2106 and sodium alginate suspension (SAS) expressed as the difference in reduction versus the controls. Higher values indicate a greater reduction in EBD absorption. The data, expressed as a column chart, represent the mean ± standard deviation (SD) (vertical bars). Paired and unpaired Student’s t-test (parametric data).

Evaluation of EBD Penetration in Epifluorescence Microscopy

To evaluate the depth of mucosal penetration of the dye, mucosal samples were collected from all esophagi as described above and as schematized in Figure 2. The representative images obtained are shown in Figure 5.

Figure 5

Evans blue dye (EBD) mucosal penetration indicated by epifluorescence microscopy: Control sample (damaged mucosa, not treated with any topical agents and not stained with EBD) showed a very high orange background. Arrows point at EBD-related signal. (A1) An EBD-related signal was present in all layers of the multilayered squamous epithelium in the sample not treated with topical agents but stained with EBD. (A2) In the fragment treated with AL2106, the background signal was very high, but the EBD-related signal was restricted to some superficial epithelium layers. (B1) After washing, a small quantity of EBD penetrated the esophageal mucosa and submucosa. (B2) In the fragments treated with the sodium alginate suspension (SAS), the dye was present in only a few layers of the epithelium. (C1) Washing in saline partially restored the ability of EBD to penetrate the esophageal mucosa and submucosa. (C2) (bars: 200µm).

Analysis of these samples suggested that the damaged esophageal mucosa displayed a very high orange background as shown in the control samples (perfused with damaging solution, but not treated with any topical agents, and not stained with EBD) (Figure 5A1).

In the samples not treated with topical agents but stained with EBD, an EBD-related signal present in all layers of the multilayered squamous epithelium was observed; the dye penetrated, affecting the lamina propria, passing through the muscularis mucosae and reaching the submucosa (Figure 5A2).

In the fragments treated with AL2106, the background signal was very high, but the EBD-related signal showed that the penetration did not affect all the layers of the epithelium (Figure 5B1). After washing in normal saline, only a minimal quantity of EBD penetrated the esophageal mucosa and submucosa (Figure 5B2).

Conversely, in the fragments treated with SAS, the presence of dye was noted in only a few layers of the epithelium (Figure 5C1). Washing in normal saline partially restored the EBD ability to penetrate the esophageal mucosa and submucosa (Figure 5C2). It could also be noted that, in the sections in which the epithelium still had keratin, it appeared intensely fluorescent.

Discussion

The aim of the present study was to evaluate the potential barrier effect and the bioadhesive capability of the new medical device called AL2106 on the esophageal mucosa. To achieve these goals, an ex vivo porcine model was used in which the damage was induced by the perfusion of an acidic/peptic solution, and the mucosal permeability was assessed by the absorption of a vital dye.7 The porcine esophagus is considered a proper model for ex vivo studies due to the great similarities between human and porcine gastrointestinal tracts.7,12 In addition, EBD is known to bind quantitatively to albumin in vivo and in vitro; therefore, it was used as an indicator of esophageal mucosal permeability.13–15 A previous experiment with the same model showed that EBD penetration was due to the increased mucosal permeability caused by exposure to the acidic/peptic solution since the intact mucosa did not absorb the dye.7 After perfusion with the damaging solution, all the untreated mucosal samples absorbed the EBD while the absorption of EBD was reduced when the esophagi were pre-treated with protective topical agents. Unlike the Authors’ previous study, a method of extraction and quantification of the dye was used to obtain a more objective measurement of EBD absorption instead of visual analysis of the staining.

In this study, the effect of AL2106, a new medical device with high bioadherence which contains a quantity of 0.5 to 5% chondroitin sulphate, a quantity of 0.05 to 5% xyloglucan and a quantity of 10 to 70% glycerol was investigated. Chondroitin sulphate is a natural glycosaminoglycan present in all connective tissue extracellular matrices, especially in the cartilage, skin, blood vessels, ligaments and tendons, where it carries out a number of biological functions (cell proliferation, differentiation, migration, tissue morphogenesis, organogenesis, infection and wound repair).16,17 Xyloglucan is a matrix polysaccharide which is present in the cell walls of all land plants. It is a natural biodegradable high-molecular weight branched polysaccharide (hemicellulose) derived from the tamarind seed. The configuration of this polysaccharide gives the product a “mucin-like” molecular structure, thus conferring optimal mucoadhesive properties. Xyloglucan possesses high swelling capacity, which is of great importance in initiating the bioadhesion process.18 Xyloglucan was used to increase the AL2106 adhesive capacity for its rheological profile; hypothetically, during swallowing, in which the stress on the formulation is high, the viscosity is low and AL2106 behaves like a liquid. On the contrary, when AL2106 adheres to the mucosa, the stress is null and it behaves like a solid, increasing molecular interaction and thus the viscosity.19

The reference compound was SAS, present on the market since 1987 and one of the most used medical devices for the treatment of GERD.8 It is composed of alginic acid, a linear polysaccharidic polymer distributed widely in the cell walls of brown algae; it is hydrophilic and forms a viscous gum when hydrated. Alginic acid derivatives, or alginates, act by creating a mechanical barrier which displaces the postprandial acid pocket. Due to its specific composition, it has been used to prevent the occurrence of reflux and to neutralize the acidity of the refluxate. Moreover, recent studies, both in vitro and in vivo, have shown its capacity of adhering to the esophageal mucosa and of preventing the mucosal impairment induced by the reflux components.6,20,21 In the present study, it was found that AL2106 was able to significantly reduce the amount of EBD absorbed by the damaged mucosa, an effect also shown by the reference device, and that this occurred even if the dye solution was applied after washing the mucosal fragments with saline.

To reduce the variability among the 19 esophagi examined and to better compare the two treatments, the difference between the dye absorbed after treatment and that of the corresponding untreated fragments was calculated. The entity of the variation induced by the treatments, either in unwashed or in washed fragments, was rather variable but the majority of the fragments showed a reduction in dye absorption ≥ 50%.

The persistence of a barrier effect after saline washing was particularly interesting since it could have represented a property displayed during more physiological conditions (ie during swallowing and salivation), therefore reflecting a critical role for the bioadhesive capability of the product.

Microscopic evaluation revealed that a damaged esophageal mucosa displayed great autofluorescence; however, it was possible to detect an EBD-related signal. In the samples not treated with any topical agents and stained with EBD, the dye penetrated the mucosa, affecting the lamina propria, passing through the muscularis mucosae and reaching the submucosa. In the samples treated with both AL2106 and the reference topical agent, the EBD signal was restricted to only some of the more superficial epithelial layers. A very high background signal was noted in the fragments treated with AL2106, probably due to some intrinsic properties of the specific formulation. Washing in saline did not seem to alter EBD distribution markedly, even if sporadic EBD-related signals were present in the submucosa and an additional increase in the background was observed. Even if the microscopic observation seemed to support the above-mentioned quantitative data, it is important to note that this type of analysis is widely influenced by both the operator and the sample tract analyzed.

Conclusion

In conclusion, in our experiments AL2106 showed a barrier protective effect on the esophageal mucosa similar to that of the topical agent used as reference and maintained its effect even after mucosal washing, thus suggesting superior resilience. Additional experimental and clinical studies may support its use as a valuable medical device for the treatment of GERD.