The present invention relates to a method for extracting aldehydes from the adhesive used for gluing needles to syringes, and to a method for determining the aldehydes releasable from said syringes, before or after such a treatment.
The development of protein-based medicaments poses major problems of contamination due to the interaction with the primary containers (e.g., syringes) in which they are placed for storage and subsequent administration. Such problems are described for example in paragraphs [0001-0007] of US20160251261A1 and in the article by Denfeng Liu et al., “Interactions between Therapeutic Proteins and Acrylic Acid Leachable,” PDA J. Pharm. Sci. And Tech. 2012, 66, 12-19.
A particular class of substances which react negatively with such drugs, and which can be released from the primary container, are aldehydes, in particular formaldehyde and acrolein (but also acetaldehyde and methacrolein), which can be present in the syringe cone due to the adhesive used to attach the needle to the syringe, and released therefrom, in particular due to the interaction with some drugs.
Various methods of decreasing the release of substances from the glues used in syringes are known.
For example, it is known to appropriately vary the emission parameters (wavelength, type of light source, time profile and radiation intensity) used during the glue curing step.
However, such methods tend not to be specific, i.e., they have no particular effect with respect to the reduction of aldehydes, and moreover, when it comes to the reduction of such extractable classes to very low levels, such methods are not sufficiently stable.
It is also known to use autoclave treatments on primary containers, for the purpose of the sterilization thereof. Such a treatment is described in EP3496765A2, for example. However, such a process is generally not suitable for syringes as it can weaken the gluing seal of the needle or damage any rubber components (such as the piston or the needle shield cap) already pre-assembled on the syringe. Accordingly, EtO gas sterilization is preferred for this type of component.
In order to keep the syringe production process under control, it is also important to develop an aldehyde detection method which is capable of determining the presence thereof irrespective of the drug later introduced therein. Such a method must be highly precise and sensitive. It is known to use liquid chromatography as a detection method, but the results obtained depend on many factors, including the substance used for the so-called aldehyde derivatization.
In fact, aldehydes are not detectable per se at low concentrations (ng/mL) if they are not first bound to a substance which allows the discrimination thereof, forming a chromophore product (hydrazone) therewith which is determinable with a simple UV-Vis detector; such a chemical process is referred to as derivatization and allows determining the aldehydes at picomole levels with a significant increase in the detectability limits.
The choice of the derivatization agent also affects the sensitivity of the method; for example, some substances do not allow detecting very small amounts of aldehydes (of the order of ng/ml), because the derivatization yields are insufficient for producing an amount of product the signal of which can be determinable even with the most modern analytical techniques.
An example of an unsuitable binder is pentafluorobenzyl hydroxylamine (PFBHA). Although the reactivity of this molecule with carbonyl groups to generate oximes is known, the development of the reaction is analyte-specific. The determination of an aldehyde reacting with PFBHA is generally possible by a mass spectrometry detector, but the derivatization reaction in this case is very sensitive to the following variables: reaction time, temperature, pH, and reagent amount for each specific aldehyde. The effect of each variable is specific to each aldehyde and makes the overall efficiency of the reaction favorable for some aldehydes but simultaneously unfavorable for others. Therefore, using this derivatization reagent does not allow simultaneously determining the four aldehydes under investigation at ng/mL concentration levels.
Furthermore, it has been found that when the tests are performed by filling the syringe with a sample liquid, such as water, the amount of aldehydes detected is also affected by other factors not dependent on the amount and quality of adhesive present in the cone, such as aldehydes present in the plunger or in the water itself.
Based on the above, it is therefore necessary to develop a syringe production method which minimizes the release of aldehydes, without causing a worsening in the release of other substances, and which is independent of the type of drug with which the syringe is filled.
There is also a need to develop an analytical method for the determination of residual aldehydes releasable by a syringe, in particular a syringe subjected to a method for extracting aldehydes from the glue.
The first technical problem set forth above is substantially solved by a method for extracting residual aldehydes from syringes comprising the technical features set forth in one or more of the appended claims, the definitions of which form an integral part of the present description for the purpose of sufficiency of description. Therefore, the present invention relates to a method for extracting residual aldehydes from syringes comprising a step of treating said syringes at a temperature higher than or equal to 50° C., preferably higher than or equal to 90° C.
The invention further relates to an analytical method for detecting residual aldehydes releasable from a syringe, the method comprising the following steps:
Further features and advantages of the invention will become apparent from the following description of preferred embodiments, given by way of non-limiting example.
In a first aspect, the present invention relates to a method for extracting residual aldehydes from syringes comprising a step of treating said syringes at a temperature higher than or equal to 50° C., preferably higher than or equal to 90° C.
The term “syringe” or “syringes” within the meaning of the present invention means a syringe-needle assembly, in which the needle is coupled to the cone of the syringe by means of an adhesive or glue containing residual aldehydes and in which the syringe does not comprise rubber parts. This glue is typically of the UV-radiation cross-linkable type.
Referring to
In certain embodiments, the pre-assembly step a) is preceded by a plasma treatment under oxygen atmosphere on the needle 3 to be glued. Such a treatment increases the wettability and surface energy of the needle 3, causing a better cleaning of the surface and therefore making it less prone to release contaminants upon gluing, possibly due to the reaction of the material of the needle with the glue.
The method for extracting residual aldehydes from syringes according to the invention comprises, as mentioned, a step of treating said syringes at a temperature higher than or equal to 50° C., preferably higher than or equal to 90° C.
Such a treatment step can be carried out under vacuum, at atmospheric pressure in a liquid or gaseous fluid or under vapor pressure. Alternative methods can be:
A particularly preferred method comprises a step of treating the syringe at a temperature between 110° C. and 130° C. and at a water vapor pressure between 1.2 and 3 bar. More preferably, the temperature is between 118° C. and 123° C. and the pressure is between 1.8 and 2.3 bar.
The treatment time is an important parameter, as times of 60 minutes or more, or 90 minutes or more, do not make significant improvements, but tend to worsen the tensile strength of the needle, or even cause it to detach already in the absence of load. The treatment time is thus between 5 and 50 minutes, or between 15 and 40 minutes, or between 15 and 25 minutes, or between 20 and 35 minutes, or between 25 and 30 minutes.
Therefore, a syringe obtainable by the method of the invention and having a releasable aldehyde content as follows forms a second object of the invention:
The evaluation of the content of aldehydes released from the syringes was carried out by a method developed by the current inventors and forming a further object of the present invention.
Such a method will be described below.
The analytical method of the invention comprises the following steps:
The sample preparation step i) comprises detaching, by means of a shear or other suitable tool, for example, the cone 2 from the cylindrical body of the syringe 1 and removing the protruding part of the needle 3. The portion of syringe 1 thus obtained, consisting of the cone 2, the portion of needle 3 inside the cone 2 and the glue 4 contained therein, further undergoes a crushing treatment of said syringe portion to give said sample.
The sample derivatization treatment step ii) comprises the steps of:
The derivatization treatment allows transforming the aldehydes released by the glues into hydrazones by reaction with the compound of formula Ar—NH—NH2. Such hydrazones are easily detectable by means of UV spectroscopy.
Preferably, said solution of water/acetonitrile/derivatization solution comprises 16-17 parts by volume of water, 1.5-2.5 parts by volume of acetonitrile, and 0.8-1.2 parts by volume of derivatization solution.
The derivatization solution comprises said compound of formula Ar—NH—NH2, where Ar is a phenyl substituted by one or more electron-withdrawing groups, and preferably consists of 120-130 parts by weight of said compound of formula Ar—NH—NH2 in 13-17 parts by volume of acetonitrile, 18-22 parts by volume of a strong acid, preferably 37% hydrochloric acid, and water to a total of 100 parts by volume.
It is important that the pH of the solution is between 1 and 1.2, more preferably about 1.1.
The compound of formula Ar—NH—NH2 is more preferably 2,4-dinitrophenyl hydrazine.
In certain embodiments, it can be necessary or advisable to crystallize 2,4-dinitrophenyl hydrazine prior to use, for example by crystallizing 2,4-dinitrophenyl hydrazine through hot solubilization in acetonitrile and subsequent reprecipitation.
Step iii) of analyzing the solution of a sample resulting from step ii), containing hydrazones of the aldehydes released by the glue in said solution, comprises the steps of:
The eluent preferably consists of a varying composition mixture of eluent A (H2O/THF 71-74%/26-29% (V/V)) and eluent B (acetonitrile).
Preferably, the operating conditions of the column are as follows:
The calculation of the residual amount of aldehydes is carried out by applying the following equation:
C
sample=(Asample×Cstandard×F×D×R)/Astandard
It has been shown that the choice of 2,4-dinitro-phenyl-hydrazine for derivatization leads to very satisfactory results.
The method thus defined has a specificity, that is, an ability to discriminate the substances sought with respect to noise, in accordance with the validation standards required by the main pharmacopoeias.
The quantification limit of the method thus exposed is highly low, and thus adapted to detect even minimal amounts of aldehydes present in the samples analyzed; the lowest quantifiable signal with respect to background noise was around 1-2 ng/ml per syringe.
The coefficient of variation (RSD×100, where RSD=relative standard deviation given by SD/mean) of the measurements according to the method of the invention is less than or equal to 3%.
The method is also stable within 10% with respect to a sample storage time of 2h at room T, or 6h at 5° C.
Table I below summarizes the tests conducted on uncapped syringes using the various aldehyde reduction methods described above. The determination of the amount of residual aldehydes was carried out as described above. In all the cases, Loctite® AA 3345, produced by Henkel, Duesseldorf was used as a glue. The test was carried out on 5 syringes for each type of treatment and the mean value of residual aldehydes±S.D. was calculated.
Treatment 1 was also repeated on capped syringes in which a rubber part is present (treatment 7).
The above data show that the 3-hour ultrasonic bath at 75′ and the autoclaving at 121° C., in particular by reducing Lle time from 60 minutes to 20 minutes, provide the best reduction of aldehyde content.
Treatments 4 and 6, while resulting in a good reduction of formaldehyde and acetaldehyde, do not provide a sufficient reduction of acrolein (particularly critical component) when compared to methods 1 and 2 in an autoclave. Furthermore, they require too long processing times for an industrial implementation thereof.
The information related to the comparison of the data in autoclave at 121° C. for 20 minutes with (treatment 1) and without (treatment 7) cap deserve particular discussion.
These data indicate that the cap, which has rubber parts, significantly contributes to the release of aldehydes. The sterilization in an autoclave without the presence of rubber parts is thus improved.
It should be noted that the removal of rubber parts to prevent a possible adhesion of the cap to the needle at high temperature due to the softening of the rubber would not be necessary per se, since the materials used f cap, including the rubber, are made to resist without “stitching” at the sterilization temperatures in the autoclave, a treatment often used by many manufacturers. However, the present inventors have verified that sterilizing in an autoclave with the cap leads to higher aldehyde contamination of the cone, since the material of the cap contains many more aldehydes, and tends to release them even in the cone, as well as in the autoclaving environment (where they are removed).
This results in a syringe which retains, even downstream of the autoclave, a higher content of aldehydes.
By autoclaving the syringe alone, the aldehydes in the syringe are then removed in a more effective manner. On the other hand, the cap, when assembled after autoclaving, does not contribute to the contamination of the syringe by aldehydes, as the contact surface between the cap and the drug is limited to the circular area related to the needle cannula and there is a blast of air between the rubber and the drug.
It is apparent that only some particular embodiments of the present invention have been described, to which those skilled in the art will be able to make all changes required to adapt it to particular applications, without departing from the scope of protection of the present invention.
Number | Date | Country | Kind |
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102021000007832 | Mar 2021 | IT | national |
102021000007835 | Mar 2021 | IT | national |
Filing Document | Filing Date | Country | Kind |
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PCT/IB2022/052317 | 3/15/2022 | WO |