OPTIMIZED METHOD FOR DECONTAMINATING PRODUCTION OF GLUCOSE POLYMERS AND GLUCOSE POLYMER HYDROLYZATES
20230279455 · 2023-09-07
Inventors
- Pierre Lanos (La Bassee, FR)
- Sophie DUVET (Quesnoy Sur Deule, FR)
- Thierry DUPONT (Vendin Les Bethune, FR)
- Fabrice Allain (Lille, FR)
- Mathieu Carpentier (Saint Andre lez Lille, FR)
- Agnes Denys (Lille, FR)
- Hela Hacine-Gherbi (Villeneuve d'Ascq, FR)
Cpc classification
C12Y302/01078
CHEMISTRY; METALLURGY
C08B37/0024
CHEMISTRY; METALLURGY
C08B37/0009
CHEMISTRY; METALLURGY
G01N33/6863
PHYSICS
International classification
C12P19/14
CHEMISTRY; METALLURGY
C08B37/00
CHEMISTRY; METALLURGY
Abstract
The present invention relates to a method for decontaminating glucose polymers or the hydrolysates of the pro-inflammatory molecules thereof. Said method includes a) providing glucose polymers or the hydrolysates thereof, b) optionally, detecting or assaying the pro-inflammatory molecules in the glucose polymers or the hydrolysates thereof provided in Step a), and c) carrying out the following purifying steps: i. treatment using an enzymatic preparation having detergent properties and clarification properties; ii. treatment using a pharmaceutical-grade activated carbon with very high adsorption properties and “micropore” porosity; iii. optionally, treatment using a second activated carbon with “mesopore” porosity; iv. passing them over a macroporous adsorbent polymer resin having porosity greater than 100 Angstroms; and v. continuous ultrafiltration at 5 kDa.
Claims
1-7. (canceled)
8. A method for decontaminating glucose polymers or the hydrolyzates thereof of the pro-inflammatory molecules thereof, comprising the following steps: a) providing glucose polymers or hydrolyzates thereof, b) optionally, detecting or assaying the pro-inflammatory molecules in the glucose polymers or hydrolyzates thereof provided in step a); and c) carrying out the following purification steps in the following order: i) treating with an enzymatic preparation with detergent and clarifying properties, ii) treating with a pharmaceutical-grade activated carbon with high adsorption capacity and microporous porosity to decrease TLR2 response, iii) treating with a second activated carbon with mesoporous porosity to eliminate molecules with a molecular weight of <100 kDa, iv) passing over a macroporous adsorbent polymer resin having a pore size greater than 100 angstrom, and v) continuous 5 kDa ultrafiltration.
9. The method as claimed in claim 8, wherein the enzymatic preparation with detergent and clarifying properties is an enzymatic preparation with mannanase activity.
10. The method as claimed in claim 8, wherein the pharmaceutical-grade activated carbon with high adsorption capacity and microporous porosity eliminates PGNs and degradation products of PGNs.
11. The method as claimed in claim 8, wherein the activated carbon with mesoporous porosity eliminates LPS and degradation products of PGNs.
12. The method as claimed in claim 8, wherein the glucose polymers are selected from icodextrin and maltodextrins, and the glucose polymer hydrolyzates are a product of total hydrolysis.
13. The method as claimed in claim 9 wherein the pharmaceutical-grade activated carbon with high adsorption capacity and microporous porosity eliminates PGNs and degradation products of PGNs.
14. The method as claimed in claim 9, wherein the activated carbon with mesoporous porosity is-eliminates PGNs and degradation products of PGNs.
15. The method as claimed in claim 9, wherein the glucose polymers are selected from icodextrin and maltodextrins and the glucose polymer hydrolyzates are a product of total hydrolysis.
16. The method as claimed in claim 8, wherein the glucose polymers are selected from branched or unbranched maltodextrins.
17. The method as claimed in claim 8, wherein the glucose polymer hydrolyzates are dextrose monohydrate.
18. The method as claimed in claim 9, wherein the glucose polymers are selected from branched or unbranched maltodextrins.
19. The method as claimed in claim 9, wherein the glucose polymer hydrolyzates are dextrose monohydrate.
20. The method as claimed in claim 8, wherein the pharmaceutical-grade activated carbon with high adsorption capacity and microporous porosity decreases TLR2 response from 80% to 10%.
21. The method as claimed in claim 8, wherein the pharmaceutical-grade activated carbon with high adsorption capacity and microporous porosity decreases TLR2 response from 65% to 10%.
22. The method as claimed in claim 8, wherein the pharmaceutical-grade activated carbon with high adsorption capacity and microporous porosity decreases TLR2 response from 100% to 10%.
23. The method as claimed in claim 8, wherein the pharmaceutical-grade activated carbon with high adsorption capacity and microporous porosity decreases TLR2 response from 60% to 5%.
Description
DETAILED DESCRIPTION OF THE INVENTION
[0085] The method of the invention is intended to replace the routes conventionally used to purify glucose polymers or the hydrolyzates thereof.
[0086] The method for decontaminating glucose polymers or the hydrolyzates thereof in accordance with the invention comprises the following steps: [0087] a) providing glucose polymers or hydrolyzates thereof; [0088] b) optionally, detecting or assaying the pro-inflammatory molecules in the glucose polymers or hydrolyzates thereof provided in step a): [0089] c) carrying out the following purification steps: [0090] i. treatment by an enzymatic preparation with detergent and clarifying properties, [0091] ii. treatment by a pharmaceutical-grade activated carbon with very high adsorption capacity and “microporous” porosity, [0092] iii. optionally, treatment by a second activated carbon with “mesoporous” porosity, [0093] iv. passing over a macroporous adsorbent polymer resin having porosity of greater than 100 angstrom, and [0094] v. continuous 5 kDa ultrafiltration.
[0095] The glucose polymers or the hydrolyzates thereof may be intended for peritoneal dialysis, enteral and parenteral feeding and the feeding of neonates.
[0096] In one preferred embodiment, the glucose polymers which will be prepared within the context of the present invention are icodextrin or maltodextrins (which are branched or unbranched, as will be described below).
[0097] The glucose polymer hydrolyzates concerned here are understood to be, especially, the product of total hydrolysis, such as apyrogenic dextrose monohydrate, sold under the trade name LYCADEX® PF by the Applicant company.
[0098] They may be decontaminated at one or several stages of their preparation, and especially at the latter steps of their preparation method.
[0099] Thus, the glucose polymers or the hydrolyzates thereof provided in the methods according to the present invention correspond to the product preceding the final product.
[0100] The pro-inflammatory components are above all molecules of bacterial origin.
[0101] They may be, in particular: [0102] PGNs, [0103] LPSs, [0104] lipopeptides. [0105] PGN depolymerization products, especially MDP, [0106] formylated microbial peptides, such as f-MLP. [0107] β-glucans, [0108] etc.
[0109] The methods for measuring the in vitro inflammatory responses which are used in the context of the present invention to monitor the effectiveness of the decontamination steps of the methods for preparing glucose polymers for therapeutic use in humans (e.g. peritoneal dialysis solutions) are based on cell tests (“bio-assays”) using lines of monocyte/macrophage type (THP-1, and/or Raw-Blue™) and transfected lines expressing a specific natural immunity receptor (HEK-Blue™), which cell tests were developed by the Applicant company and detailed in its prior patent applications.
[0110] Five lines are preferably used: [0111] Raw-Blue™ line: this line, derived from mouse macrophages, responds to the majority of the pro-inflammatory contaminants that may be present in the glucose polymer matrices and derivatives (PGN, lipopeptides, LPS, zymosan. LTA). Its use therefore makes it possible to estimate the overall load of pro-inflammatory molecules present in the samples. [0112] HEK-Blue™ hTLR2 line: this line, expressing the hTLR2 receptor, specifically responds to TLR2 agonists (PGN and lipopeptides above all). Its use therefore makes it possible to determine the level of these contaminants in the triggering of inflammatory responses. [0113] HEK-Blue™ hTLR4 line: this line, expressing the hTLR4 receptor, specifically responds to LPSs. Its use therefore makes it possible to determine the level of these contaminants in the triggering of inflammatory responses. [0114] HEK-Blue™ hNOD2 line: this line, expressing the hNOD2 receptor, specifically responds to NOD2 agonists. Its use therefore makes it possible to determine the level of MDP and related molecules in the triggering of inflammatory responses. [0115] HEK-Blue™ Null2 line: this is a control line which has not been transfected with an immunity receptor. Its use is necessary to verify that the solutions of glucose polymers or of hydrolyzates thereof do not induce SEAP production via a toxicity mechanism.
[0116] However, it should be noted that those skilled in the art may also use other commercial lines (IMGENEX) or they may prepare them.
[0117] In one preferred embodiment, the cell lines are used at a density between 0.5 and 1×10.sup.6 cells/ml of culture medium, and the bringing of the preparation of glucose polymers or hydrolyzates thereof into contact with the cells lasts approximately 16 to 24 h.
[0118] Quantification of the contaminants may be carried out using a dose-response curve. This dose-response curve may especially be produced with the same cells, under the same conditions, with increasing doses of contaminants. The dose-response curves are in particular produced with LPS, PGN, lipopeptide and MDP standards.
[0119] Preferably, such a dose-response curve can be produced for cons expressing TLR4 (for example, THP-1. HEK-Blue™ hTLR4 and Raw-Blue™) with increasing doses of LPS, for cells expressing TLR2 (for example. THP-1, HEK-Blue™ hTLR2 and Raw-Blue™) with increasing doses of PGN, and for cells that are reactive via NOD2 (for example, HEK-Blue™ hNOD2) with increasing doses of MDP.
[0120] The cell tests may be carried out as described in the Applicant's patent applications: WO2012/143647 and WO2013/178931.
[0121] The first decontamination step of the method in accordance with the invention consists of a treatment by an enzymatic preparation with detergent and clarifying properties.
[0122] This enzyme activity of mannanase type, such as the enzymatic preparation Mannaway® sold by Novozymes, has proven effective for dissociating macro complexes such as bacterial debris and high molecular weight PGNs.
[0123] Its activity is optimal when it is used at a final concentration of 0.4% (vol/vol) In the 32% (weight/vol) glucose polymer solution, adjusted to pH 10 with NaOH, for a treatment time of 24 h at 50° C.
[0124] After treatment, the solution is neutralized by HCl and the enzyme is inactivated by heating at 85° C. for 10 mins.
[0125] The second step consists of a treatment by a pharmaceutical-grade activated carbon with very high adsorption capacity and “microporous” porosity.
[0126] The Applicant company recommends using an activated carbon of Norit C Extra USP type. This is because C Extra USP carbon proves effective in eliminating PGNs and their degradation products.
[0127] Its activity is optimal when it is added at the final concentration of 0.5% (weight/volume) in the 32% (weight/vol) glucose polymer solution, adjusted to pH 4.5 with HC. The treatment is carried out under stirring for 1 h at 80° C. After treatment, the solution is neutralized by NaOH then filtered through 0.22 μm.
[0128] The third step consists of a treatment by a second activated carbon with “mesoporous” porosity. This step is optional.
[0129] Here, an activated carbon of ENO-PC type is preferred. This quality of activated carbon has a broad spectrum of action and makes it possible preferentially to eliminate molecules with a molecular weight of <100 kDa (for example, LPS and degradation products of PGNs).
[0130] It is also used here at a content of 0.5% at pH 4.5 for 1 h at a temperature of 80° C.
[0131] The fourth step consists of a treatment on a macroporous adsorbent polymer resin having a porosity of greater than 100 angstrom.
[0132] Dowex SD2 resin is chosen, which has a broader spectrum of elimination of contaminating molecules (other than PGNs) than other resins of the same family.
[0133] The 32% (250 ml) glucose polymer solutions are eluted on a column containing 20 ml of this resin.
[0134] The final step consists of filtration on an ultrafiltration membrane having a cut-off threshold of 5 kDa.
[0135] The aim of the treatment by ultrafiltration is to eliminate the molecules of small size that are still present in the glucose polymer solutions. The Applicant company recommends using this treatment at the end of the method, since this treatment also has a dialysis effect which makes it possible to eliminate traces of salts which have accumulated over the course of the preceding treatments.
[0136] It is chosen to continuously inject the glucose polymer solution over a 5 kDa filter at a rate of 25 ml/min for 3 h at room temperature. To compensate for the loss of filtrate, the retentate is injected into the starting solution and continually adjusted to the initial volume (100 mi) by addition of sterile PBS buffer. After 3 h, the volume of filtrate is between 150 and 200 ml, which is greater than the initial volume of the glucose polymer solution.
[0137] As will be shown in the examples below, this combination of steps alone is able to provide maximum protection for the circuits for producing polymers and glucose and derivatives thereof from contaminants of bacterial origin.
[0138] The invention will be understood more clearly from the following examples which are intended to be illustrative and nonlimiting.
EXAMPLES
Example 1: Establishment of the Dose-Response Curves
[0139] The dose-response curves are produced with standard agonist molecules: LPS, PGN, PAM3(cys) (PAM.sub.3Cys-Ser-(Lys)4 trihydrochloride, a synthetic lipopeptide), LTA, zymosan and MDP. The Raw-Blue™ and HEK-Blues™ hTLR2, hTLR4, hNOD2 and Null lines are incubated with increasing concentrations of agonists, and the cell response is measured by quantifying the SEAP activity. TNF-α is used as positive control for cell activation: [0140] Raw-Blue™ line (
Example 2: Preparation of the Various Glucose Polymer Matrices
[0145] As Indicated above, the matrices are as follows: [0146] 4 glucose polymers, raw materials of icodextrin (before chromatographic fractionation according to the teaching of patent EP 667 356), referenced here E1565, E3063, E1242 and E5248
[0147] The preparation of these polymers is carried out in accordance with the teachings of patent application WO 2012/059685; [0148] a contaminated batch of icodextrin (referenced here E209J) and a “negative control” batch of icodextrin, i.e. control for non-contamination in the cell tests (referenced here P11-11). These batches are prepared according to the teaching of patent EP 667 356, described in detail in example 1 of patent application WO 2010/125315.
Example 3: Analysis of the Cell Responses Induced by the Untreated Samples
[0149] The aim of these tests is to determine the pro-inflammatory reactivity and the nature of the contaminants present in the various matrices.
[0150] The samples according to example 2 are prepared at 32% (weight/volume) in non-pyrogenic water (or injection).
[0151] The assays of the LPS and PGN levels were carried out prior to the cell tests using the SLP-HS and LAL assays (data presented below):
TABLE-US-00001 P11- 11 E1242 E1565 E3063 E5248 E209J SLP-HS <3 21 2320 16185 116 393 PGN (ng/g) LAL LPS (EU/g) <0.3 2.4 38.4 2.4 9.6 0.6 Modified LAL <0.3 1.2 4.8 1.2 0.3 <0.3 LPS (EU/g)
[0152] The presence of biocontaminants in the various matrices was analyzed by means of the five cell types, so as to have an overview of the inflammatory responses to certain contaminants (
[0153] For the cell tests, the samples are diluted to 1/10 in the cell culture medium (final concentration: 3.2% (w/v)).
[0154] The analyses are carried out on: [0155] Raw-Blue™ line: any contaminants with high reactivity for PGNs, [0156] HEK-Blue™ hTLR2 line: high reactivity for PGNs and lipopeptides, [0157] HEK-Blue™ hTLR4 line: high reactivity for LPSs, [0158] HEK-Blue™ hNOD2 line: MDP and PGN depolymerization products, [0159] HEK-Blue™ Null2 line: control for absence of cell toxicity.
[0160] Assessment by sample: [0161] E1242: high-intensity inflammatory response in the HEK-TLR2 cells, and low-Intensity Inflammatory response in the HEK-NOD2 cells, evidence of a strong contamination with barely degraded PGNs. [0162] E1585: high-intensity inflammatory response in the HEK-TLR2 cells, medium-intensity inflammatory response in the HEK-TLR4 cells and very high-intensity inflammatory response in the HEK-NOD2 cells, evidence of a strong contamination with degraded PGNs and with LPSs. [0163] E3063: saturated inflammatory response in the HEK-TLR2 cells, medium-intensity inflammatory response in the HEK-TLR4 cells and low-intensity inflammatory response in the HEK-NOD2 cells, evidence of a very strong contamination with barely degraded PGNs and with traces of LPSs. [0164] E5248: low-Intensity inflammatory response in the various lines, evidence of a low contamination with PGNs and with LPSs. [0165] E209J: high-intensity inflammatory response in the HEK-TLR2 cells, and low-intensity inflammatory response in the HEK-NOD2 cells, evidence of a strong contamination with weakly degraded PGNs.
[0166] None of the glucose polymer matrices gives a response in the presence of HEK-Null cells, which confirms the absence of cytotoxicity.
Example 4: Analysis of the Effect of the Decontamination Procedures on the Cell Responses Induced by the Samples
[0167] In its International patent application WO 2013/178931, the Applicant company enabled identification of the treatments best suited to each type of contaminants present in the samples, and made it possible to determine the experimental conditions for their application to glucose polymer matrices.
[0168] On the basis of this earlier study, the numerous individual treatments proposed are: [0169] treatment over activated carbon, [0170] ultrafiltration through a membrane with a 5 kDa filtration threshold, [0171] passage over adsorption resins, [0172] treatment by enzymatic preparations.
[0173] In the experiments with the combinations described below, the choice and the arrangement of the steps was determined as a function of [0174] the experimental treatment conditions, [0175] the levels of contamination in the samples, and [0176] the nature of the pro-inflammatory molecules.
[0177] Use of Mannaway®
[0178] The teachings of International patent application WO 2013/178931 showed that the enzymatic preparation is slightly contaminated by traces of LPS. In addition, traces of enzyme may persist after treatment in the glucose polymer solution. So as to eliminate these exogenous contaminations, the Applicant company therefore recommends placing the enzymatic treatment step at the start of the procedure in the tests of combinations.
[0179] Use of Activated Carbons
[0180] The activated carbons retained for the present study are: [0181] C EXTRA USP, for its effectiveness in eliminating PGNs and their degradation products; [0182] ENO-PC, for its preferential action on contaminants of molecular weight <100 kDa (for example, LPS and degradation products of PGNs); [0183] A SUPRA EUR, for its effectiveness in eliminating complexes of high molecular weight.
[0184] The Applicant company has chosen to use the activated carbons alone or combined in pairs in the various combinations, and given that the treatments by carbons are carried out batchwise and require heating, neutralization and filtration steps, they are carried out just after the enzymatic treatment but before the other treatments.
[0185] Use of Resins
[0186] The resins retained are: [0187] Macronet MN-150, for its effectiveness in retaining molecules of low molecular weight (for example MDP and degradation products of PGNs); [0188] Dowex SD2, for its broad spectrum of elimination of contaminants, except PGNS.
[0189] Use of Membrane Separation
[0190] The aim of the treatment by 5 kDa ultrafiltration is to eliminate the molecules of small size that are still present in the glucose polymer solutions. In addition, this procedure has a dialysis effect and makes it possible to eliminate traces of salt that have accumulated over the course of the previous treatments.
[0191] This step is therefore systematically placed at the end of the procedure.
[0192] After each step, samples are taken under sterile conditions and are used in the cell tests, so as to assay the overall inflammatory load (Raw-Blue™ cell response) and the amounts of blocontaminants (HEK-Blue™ responses). The cell responses obtained after each step are compared to the response induced by the starting matrix, so as to estimate the effectiveness of the decontamination procedures. The results are expressed as activity relative to the maximum cell response. In all the tests, a non-contamination control is carried out with a solution of P11-11 icodextrin.
Example 5: Comparative Analysis of Various Combinations of Individual Treatment Steps
[0193] A large number of possible combinations may be implicitly deduced from the teaching of patent application WM 2013/178931.
[0194] The results obtained for 3 of the conceivable procedures are as follows.
[0195] Procedure 1: E1242 Matrix: Treatment by C EXTRA USP+ENO-PC Activated Carbons: Passage Over Macronet MN-15 Resin: 5 Da Ultrafiltration
[0196] The results of the cell tests are given in
[0197] The E1242 matrix induces an intermediate inflammatory response in the Raw-Blue calls, which is predominantly linked to a high concentration of PGN (TLR2 response).
[0198] It also contains traces of LPS and of degradation products of PGNs, given that the TLR4 and NOD2 responses are close to background noise.
[0199] The decontamination procedure effectively reduces the inflammatory responses.
[0200] Nonetheless, the response of the Raw-Blue cells remains slightly higher than the non-contamination control (P11-11), indicating that traces of contaminants are still present.
[0201] This result is due to the presence of residual PGNs after decontamination.
[0202] Indeed, the TLR2 response is greatly reduced after treatment by the carbons, but remains higher than the negative control.
[0203] The other steps do not have an effect on the TLR2 response, which does not evolve any more up to the end of the procedure. On the other hand, the TLR4 response is no longer detectable as early as at the 1.sup.st treatment step, which proves that the LPSs have been eliminated. Regarding the NOD2 response, this is suppressed after the ultrafiltration step.
Conclusion
[0204] Although the load of inflammatory compounds has been reduced effectively, procedure 1 Is insufficient to ensure complete decontamination of a matrix heavily loaded with PGNs.
[0205] Procedure 2; E209J Matrix: Treatment by C EXTRA USP+ENO-PC Activated Carbons: Passage Over Dowex SD2 Resin: 5 kDa Ultrafiltration
[0206] The results of the cell tests are given in
[0207] For this procedure, the resin was replaced by Dowex SD2, which has a broader spectrum of retention. The tests were carried out with the E209J matrix, which has a contamination profile similar to that of E1242.
[0208] In this case, the response of the Raw-Blue cells is identical to the negative control, which proves that decontamination has been effective.
[0209] Nonetheless, the TLR2 response is still higher than the non-contamination control, which indicates that traces of PGN are still present.
[0210] The difference in the responses is certainly linked to the fact that the HEK-TLR2 cells have a lower detection threshold for PGNs than the Raw-Blue cells.
[0211] The NOD2 response is reduced after passage over SD2 and suppressed after ultrafiltration, which suggests that this resin has an at least complementary action to eliminate the degradation products of PGNs.
Conclusion
[0212] This data indicates that the change in resin has not improved the effectiveness of the procedure in eliminating all the PGNs.
[0213] Procedure 3: E5248 Matrix: Treatment by Mannaway® then by C EXTRA USP+A SUPRA EUR Carbons: Passage Over Dowex SD2 Resin: 5 kDa Ultrafiltration
[0214] The results of the cell tests are given in
[0215] In this final combination, A SUPRA EUR carbon was combined with C EXTRA USP as replacement for ENO-PC.
[0216] Contrary to the latter, A SUPRA EUR carbon preferentially eliminates molecules of high molecular weight.
[0217] This combination should be effective for decontaminating samples loaded with aggregated macro complexes of PGN or p-glucan type.
[0218] The tests were carried out on the E5248 matrix, which induces a low-intensity inflammatory response in the various lines, while assays of SLP-HS and LAL suggest the presence of a strong contamination of PGN and/or p-glucans.
[0219] This difference may be explained by the high mass of the inflammatory molecules, which would reduce their solubility, and consequently their accessibility inducing a response in the test cells.
[0220] After the 1.sup.st step of the procedure, a strong increase in cell responses is observed in the various lines.
[0221] This result confirms that the enzymatic treatment by Mannaway® is effective in disaggregating bacterial complexes or debris, thereby releasing agonist molecules for TLR2, TLR4 and NOD2.
[0222] After treatment with the carbons, the responses of the Raw cells and the HEK-TLR2 cells have decreased significantly but remain above the negative control.
[0223] Likewise, the TLR4 and NOD2 responses remain large, and it is necessary to await the passage over the resin and the final step of ultrafiltration to obtain a signal identical to the non-contamination control in the various cell types.
Conclusion
[0224] These results indicate that A SUPRA EUR carbon has not provided any notable benefit to the decontamination procedure.
Final Conclusion
[0225] Although entirely conceivable, none of these decontamination procedures gives an entirely satisfactory result.
Example 6: Presentation of the Optimized Procedure
[0226] It is chosen to carry out the succession of the following steps on the E3063 matrix.
[0227] treatment by Mannaway®, then [0228] by C EXTRA USP+ENO-PC activated carbons, then [0229] passage over Dowex SD2 resin, and finally [0230] 5 kDa ultrafiltration.
[0231] The results of the cell tests are given in
[0232] To increase the effectiveness of the procedure aiming to eliminate PGNs, a step of enzymatic treatment by Mannaway® Is introduced upstream of the other steps.
[0233] For these tests, the E3603 matrix, which is very heavily loaded with PGNs, was used.
[0234] After the various steps of the procedure, the response of the Raw-Blue cons is identical to the negative control, which proves that decontamination has been effective.
[0235] In addition, the combination of enzyme+carbon treatments is particularly-suited to eliminating PGNs, since the TLR2 response goes from a saturated signal before treatment to a signal identical to the non-contamination control.
[0236] Finally, the other steps are effective in eliminating traces of LIPS (TLR4 response) and NOD2 agonists.
[0237] In order to demonstrate that this combination is indeed effective, the ENO-PC carbon was removed so as to verify whether is use really provides a benefit to the decontamination procedure.
[0238] The results of the cell tests are given in
[0239] The tests were carried out on another matrix. E1565 matrix, which is contaminated with the various agonists of TLR2, TLR4 and NOD2.
[0240] At the end of the procedure, the response of the Raw-Blue cells has decreased significantly, but remains slightly greater than the non-contamination control. This very weak response is not linked to the presence of residual PGN but rather to traces of IPS and of NOD2 agonists, and to a possible synergistic effect between the two families of molecules.
[0241] The ENO-PC carbon has a broad spectrum of retention for molecules of molecular weight <100 kDa (LPS and degradation products of PGNs).
Conclusion
[0242] It is observed that its absence has reduced the effectiveness of the decontamination procedure, especially if the matrix is heavily contaminated with these two families of inflammatory molecules.
[0243] Altogether, the results obtained in this study show that the combination of several decontamination steps carefully selected and placed in order proves effective in eliminating the inflammatory molecules that may be present in the glucose polymer solutions.
[0244] The combination comprises the following steps: [0245] treatment by an enzymatic preparation with detergent and clarifying properties, for example Mannaway®, [0246] treatment by an activated carbon of porosity equivalent to C EXTRA USP, [0247] optionally, treatment by a second activated carbon of porosity equivalent to ENO-PC for matrices loaded with degraded PGNs and/or LPS, [0248] passage over an adsorption resin of Dowex-SD2 type. [0249] continuous 5 kDa ultrafiltration.
[0250] The steps selected make it possible to target the various families of contaminants and to propose products devoid of inflammatory reactivity.
FIGURES
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