FR2555074A1 - Device for separating blood and obtaining serum - Google Patents

Abstract

The invention relates to a device for separating blood, being in the form of a plastic or glass tube, characterised in that: - its internal walls are coated with a film-forming skin consisting of a vinyl pyrrolidone/vinyl acetate copolymer; - it contains microspheres of a styrene polymer including, on their surface, micronised hydrated silica. o

Description

Device for separating blood and obtaining serum.

 The present invention relates to a process for the separation of blood which in particular makes it possible to activate the production of human or animal serum.

 It is well known that, for the purposes of analysis of the components of human and animal blood, it is necessary to separate the blood, in particular by coagulating it. This coagulation must however be carried out in a very rapid, neutral, fibrin-free, safe and effective manner, without deterioration of the components of the blood and it is necessary to avoid hemolysis thereof.

 A number of devices are already known which make it possible to separate the coagulated blood into a light phase formed essentially of serum and a heavy phase formed essentially of cellular and fibrillar materials.

 However, in this type of process the latent formation of fibrin in the light fraction or serum can lead to contamination of the serum by fibrin and affect the apparent chemical contents of the serum measured by the control equipment.

 The coagulation times are generally of the order of 30 minutes, which poses problems in terms of the contamination of the serum by the breakdown products of the blood.

 One of the objectives of the present invention is therefore to have a very rapid blood coagulation of less than 3 minutes, which allows an analysis of the constituents of the latter giving results very close to reality.

 In the prior art, various devices have been used, all of which have the drawback of requiring a relatively long time of coagulation.

 It was thus recommended to use plastic tubes having the advantage of a neutral contact surface but very significantly delaying the coagulation of the blood due to the adhesion of red blood cells on the walls. inner tubes.

 In addition to the disadvantage of a delay in coagulation, these tubes also often require the use of a peeling off of the clot from the walls of the tubes using a rod, which presents risks of hemolysis.

 It has also been recommended in the prior art to use glass tubes of the "soda-lime" type providing a wettable surface in contact with whole blood. These tubes also do not accelerate the coagulation of blood and most often lead to variable coagulation according to the morphology of the constituents of the blood collected.

 The nature of the glass itself presents a certain number of risks for use, due to the possibility of diffusion from the internal surfaces of certain well known components of the glass, such as for example sodium or potassium. These components, due to the fineness of the chemical or biochemical analyzes in this area, may interfere with the analyzes of the blood itself.

 It has moreover already been recommended to use glasses of neutral quality which are of a very high cost price and offer no substantial advantage with regard to the acceleration of coagulation.

 To overcome this drawback, it has been proposed to coat the walls with a silicone barrier layer compatible in terms of medico-biological analyzes. The use of this type of product, however, has a major drawback which is to further delay blood clotting.

 The present invention solves these various problems and allows ultra-rapid coagulation over time of the order of 1 to 3 minutes. It leads to obtaining a serum in a plastic or glass container, in which the possible interference is reduced to a minimum due to the absolute neutrality of the container, the absence of fibrin and of components such as calcium, potassium, iron, lack of hemolysis.

 The invention also makes it possible to have an automatic physical separation between the serum and the heavier phase formed essentially of cellular and fibrillar material.

 The object of the invention is therefore constituted by a container, preferably in the form of a tube, allowing the separation of human or animal blood and comprising internal walls coated with a film-forming layer which is not soluble in blood.

 Another object of the invention is constituted by a container in particular in the form of a tube comprising a coagulation activator constituted by silica and a serum separator constituted by microbeads.

 Other objects of the invention will appear on reading the description of the examples which follow.

The device for separating human or animal blood consists of a container, preferably in the form of a plastic or glass tube, which is characterized in that at least the internal surface of said container is coated with a non-soluble film-forming layer. in blood and chemically neutral consisting of a vinylpyrrolidone / vinyl acetate copolymer
These copolymers are known in themselves and have never been used in the context of blood separation devices. Surprisingly, they have the advantage compared to the silicones recommended to date, of having a remarkable surface activity of contact with the blood, since they make it possible to activate at the level of the internal surface of the devices and separation of clotting factors from the blood.

This film-forming film also has the advantage of constituting an effective barrier vis-à-vis in particular the constituents of glass which could possibly diffuse over time on the surface of the walls and interfere with the dosages of the constituents of the serum.
This device can of course also contain a coagulation activator known in itself or the coagulation activator described below as well as means for separating the serum such as microbeads known in themselves or of the type of those defined below
According to a variant, the blood separation device according to the invention consists of a container, preferably in the form of a plastic or glass tube, characterized in that it contains at least one coagulation activator which is silica micronized superfine hydrate.

This silica is made up of agglomerates resulting from the association of aggregates themselves constituted by enchannements of unitary particles. The average diameter of these agglomerates is around 3 microns, the diameter of the elementary particles being around 20 millimicrons, the silica used is part of the range of pigments called "silicates". This coagulation activator used in accordance with the invention has a very light and very absorbent ultrafine morphology. A particularly suitable product is that sold under the name TIXOSIL by the company Rhne
Poulenc.

 The applicant has found that the use of this product makes it possible to significantly accelerate the solidification of the clot and to minimize the formation of fibrin which remains in suspension in the serum fraction after centrifugation. The use of this activator eliminates any contamination by fibrin due to the latent transformation of fibrinogen into fibrin.

 This activator also plays a role of dispersant with regard to all the solids used in suspension in the liquid. This coagulation activator is preferably used in proportions of about 0.6 to 1 mg per tube with a capacity of 5 to 10 ml.

 It goes without saying that this coagulation activator can replace the coagulation activators used in conventional tubes insofar as it will have an action of acceleration of blood coagulation which is particularly remarkable compared to the products recommended to date such as glass, kaolin, bentonite, diatomaceous earth or kieselguhr-like substances.

This activator can also be used with conventional separation means or with the separation balls defined below which constitute another variant of the invention
According to another variant of the invention, the blood separation device consists of a plastic or glass container, preferably in the form of a tube, characterized in that it contains at least microbeads constituted by a styrenic polymer containing or not a blowing agent. These microbeads can be in the form of pearls or colorless or colored sticks. The diameters or the usable sections can vary between 0.2 and 0.8 mm.

 Pearls with a diameter of about 0.6 mm are particularly preferred because of the security they present, in particular with respect to the risks of aspiration of the balls in the lines of the devices of automatic machines or of manual micropipettes.

 The styrenic polymers used in accordance with the invention exhibit interesting physicochemical properties insofar as these polymers are inert and have remarkable stability with respect to blood and these components.

 By their choice, the styrenic microbeads in accordance with the invention also play a role of tight barrier constituting a separation between the components of the blood and in particular between the heavy phase and the light phase constituted by the serum. Indeed, the applicant has found that after centrifugation, the microbeads stabilize and constitute a tight barrier by swelling between the serum and the coagulate. This has the advantage of eliminating any possible contamination between the serum and the coagulate.

 A particularly suitable product consists of microbeads of STYROSEL or STYROPORE sold by the company BASF.

 A particularly preferred variant of the invention consists in using microbeads as defined above coated with the coagulation activator constituted by hydrated silica micronized superfine.

 The coating of the styrenic microbeads with the aforementioned silica is carried out according to conventional coating coating methods.

 A particularly preferred embodiment is constituted by a device for separating human or animal blood which is in the form of a plastic or glass container more particularly in the form of a tube closed by a plastic or rubber stopper under vacuum which is characterized in that the walls are coated with a thin layer of a vinylpyrrolidone / vinyl acetate copolymer and which contains microbeads in the form of beads of a styrenic polymer having a diameter of between 0.2 and 0.6 mm coated with superfine hydrated silica.

 The use of a device comprising these three elements in combination makes it possible to optimally solve the problems posed by blood tests and in particular the separation of serum.

 The following example is intended to illustrate the invention without, however, being limiting in nature.

 A solution for treating a tube intended for blood analysis is firstly prepared by dissolving a polyvinylpyrrolidone / vinyl acetate copolymer. This solution is applied by wetting, filling or spraying on at least the inner walls of the tube. The film-forming layer thus obtained is dried in the open air.

In a second step, microbeads are prepared by coating the coagulation activator. The process is carried out dry using 2.5 g of micronized superfine hydrated silica sold under the name TIXOSIL 375 J by the Company
Rhône Poulenc in the form of an agglomerate having an average diameter of approximately 3 microns per kg of calibrated microbeads of styrenic polymer (sold under the name STYROSEL by BASF), these microbeads having a diameter of approximately 0.6 mm. By mixing the micronized silica particles are fixed on the microbeads.

 0.25 g of microbeads coated with the micronized silica as described above are introduced into a tube with a capacity of approximately 10 ml. A rubber stopper is applied to this tube after carrying out the vacuum.

The blood is taken and it is noted at the time of the introduction of the blood into the tube that the microbeads are distributed throughout the volume thus promoting close contact between the activator and the constituents of the blood. Coagulation is complete after 2-3 minutes. Centrifugation is then carried out according to conventional methods. We thus observe in the tube, three well separated phases, comprising a first phase constituted by clear serum, a second phase constituted by very tight microbeads forming a barrier and a third phase constituted by the blood clot.

Claims (9)

 1. Device for the separation of human or animal blood in the form of a plastic or glass container, characterized in that the interior walls of this container are coated with a film-forming film consisting of a vinylpyTrolidoneVinyl acetate copolymer .  2. Blood separation device according to claim 1, charac terized in that it additionally contains as blood coagulation activator at least hydrated silica micronized superfine.  3. Device according to claim 2, characterized in that the hydrated silica consists of agglomerates having an average diameter of approximately 3 microns.  4. Device according to claim 2 or3, characterized in that approximately 0.65 mg of hydrated silica is used for a tube having a capacity of 5 to 10 ml.  5. Device according to any one of claims l to 4, characterized in that it contains in its lower part calibrated microbeads of a polymer or a styrene copolymer optionally containing a blowing agent.  6. Device according to claim 5, characterized in that the microbeads are in the form of perlas having a diameter between 0.2 and 0.8 mm.  7. Blood separation device consisting of a container made of plastic or glass, characterized in that it contains at least one coagulation activator constituted by a hydrated silica micronized superfine.  8. Device according to claim 7, characterized in that this device also contains microbeads of a polymer or copolymer of styrene having a diameter varying between 0.2 and 0.8 mm.  9. Device according to claim 8, characterized in that the microbeads are coated with micronized hydrated silica.  ] 0. Process for the separation of blood, characterized in that one introduces human or animal blood into a device as defined in any one of Claims 1 to 9, and that after coagulation one proceeds to centrifugation.