WO1980000531A1 - Allergy testing system - Google Patents
Allergy testing system Download PDFInfo
- Publication number
- WO1980000531A1 WO1980000531A1 PCT/US1979/000553 US7900553W WO8000531A1 WO 1980000531 A1 WO1980000531 A1 WO 1980000531A1 US 7900553 W US7900553 W US 7900553W WO 8000531 A1 WO8000531 A1 WO 8000531A1
- Authority
- WO
- WIPO (PCT)
- Prior art keywords
- skin
- allergens
- testing
- handle portion
- substances
- Prior art date
Links
- 238000012360 testing method Methods 0.000 title claims abstract description 57
- 206010020751 Hypersensitivity Diseases 0.000 title claims description 16
- 230000007815 allergy Effects 0.000 title claims description 16
- 208000026935 allergic disease Diseases 0.000 title claims description 14
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Classifications
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61B—DIAGNOSIS; SURGERY; IDENTIFICATION
- A61B17/00—Surgical instruments, devices or methods
- A61B17/20—Surgical instruments, devices or methods for vaccinating or cleaning the skin previous to the vaccination
- A61B17/205—Vaccinating by means of needles or other puncturing devices
Definitions
- the present invention relates to skin testing with biological substances.
- it relates to medical methods and devices for allergy detection, including intracutaneous injuction of biologicals, ' such as aeroallergens, food allergens, and other chemical substances.
- Diagnosis of allergies in the past has depended upon a number of techniques for introducing various biological substances to the epidermis or der is.
- the scratch test various allergenic sub ⁇ stances are applied by abrading or cutting the epidermal layer and contacting a liquid allergenic extract or the like with the exposed skin tissue.
- These test areas are often on the back of a human patient, who may be subject to many painful tests.
- the superficial scratches or abrasions produce a less severe reaction than dermal injection. If no response or weak responses are obtained in the scratch tests, less concentrated allergens may be applied to the upper extremities of the patient intradermaliy with a small bore needle and syringe. Reactions to these latter tests may be dramatic and even require emergency measures due to the severity of the reaction.
- scarifiers have found use in applying other biological substances. For instance, vaccinations may be effected with such devices. Antigens have been applied intradermally for the Heaf multiple puncture tuberculin test.
- the present invention provides a system for allergy testing wherein common antigens are incorporated in a plurality of injector units adapted for intracutaneous use.
- the individual injector units are intended to be supplied as part of a multiple-allergen screening and/or diagnostic kit.
- a new skin test device for intracutaneous use has been devised.
- This device is an applicator or injection unit having a hilt or flat plate portion and a hollow rigid handle portion attached to the plate portion on one side thereof and adapted for grasping the device.
- a hollow metal cannula scarifier element is mounted on the flat plate, extending outwardly from the flat plate opposite the handle portion a predetermined length for intradermal injection.
- the cannula has a sharp skin-piercing point at its lower extremity and a shaft portion extending upwardly through the flat plate into said hollow handle portion.
- This configuration permits the device to be loaded with a predetermined amount of fluent skin testing substance, which may be applied to the point by dipping and distributed into the hollow scarifier by capillary action.
- the flat plate portion and handle portion may be integrally molded of thermoplastic resin, such as polypropylene.
- the handle portion comprises an elongated cylindrical tube having an open top end, and the flat plate portion has a sleeve projecting upwardly into the hollow handle portion for holding the scarifier element firmly with a predetermined prong length exposed below the hilt.
- An allergy testing kit for multiple allergen screening may be assembled with a number of these applicators or injection units.
- a base member comprising a plurality of recessed depressions, each having a well portion adapted to receive a needle-like prong, is provided with the kit.
- a corresponding number of intracutaneous injection units adapted for being held in the recessed depression of the base member is provided, each comprising a hilt portion adapted for insertion into a complementary recessed depression of base member.
- a downwardly extending skin test prong portion is adapted for insertion into the corresponding well. The upwardly extending handle portion can be grasped manually for applying the injection units sequentially.
- At least one of the prongs is loaded with a mixture of biologically active allergens, at least one of the prongs is loaded with a histamine control substance, and at lease one of the prongs is loaded with a diluent devoid of biologically active substance.
- the assembled kit may include a sealed package of ethylene-oxide-permeable material for containing the base member and injection units, permitting sterilization after assembly.
- the test prongs comprise a hollow cannula or hypodermic needle extending from the hilt into the base well
- FIG. 1 is a perspective view of the novel applicator system, showing the base and an injection unit;
- FIG. 2 is a vertical cross-section view of an injection unit;
- FIG. 3 is a schematic view of the injection unit during use
- FIG. 4 is a vertical cross-section view of the packaged base containing an injection unit
- FIG. 5 is a partial cross-section view of an alternative embodiment
- FIG. 6 is a cross-section view of a preferred embodiment of the invention showing a modified base member with vent- means.
- a base member 10 in the form of a stable flat tray is provided with a plurality of recessed depressions 12 adapted to receive individually removable applicators or injection units 20.
- the depressions are aligned in one or more rows for ease of identification and to facilitate use cf the individual applicators.
- An enlarged sectional view of a single injection unit 20 is depicted in Fig. 2.
- a metal cannula is held firmly in the hilt portion 22 of the injection unit.
- the hilt portion comprises a flat plate, with a two-tier configuration 22, 23.
- the handle portion 25 shown as an elongated cylindrical tube may have an opening at its top end or elsewhere to permit gas access to the interior or the injection unit.
- the flat plate or hilt portion 22 of the injection unit has a sleeve 28 projecting upward into the hollow handle portion. This prevents slippage during use of the cannula 30 as a scarifier, with a predetermined length exposed below the flat plate or hilt 22, 23.
- the cannula may be dipped into the fluid, with the skin-piercing point 32 being received into a well to prevent damaging the point.
- a hollow portion 34 provides a liquid reservoir on the cannula scarifier element 30, 32.
- the injection unit 20 is removed manually from the base and inserted into the skin, as shown in Fig. 3.
- the hollow metal scarifier element 30 pierces the epidermal layer 40 and extends there through into the dermis 42, where the substance carried on the scarifier prong is deposited intracutaneously. Ordinarily, -the injection unit is withdrawn immediately after injecting the test substance.
- the base member 10 may be packaged as part of a testing kit, as shown in Fig. 4.
- the base is
- ⁇ provided with a plurality of circular depressions 12 into which the hilt portion of injection unit 20 is inserted.
- the bottom of this recessed portion is tapered downwardly to a depth of about 3mm, premitting the lower prong tip 32 to be accommodated within a well 14, which may be conoidal in shape.
- a measured quantity of the particular biological substance or diluent is placed in the bottom of the well, 14.
- a lid 18 is placed over the base member 10, preventing the individual injection units from becoming loose.
- a projecting segment 16 can be molded onto the base 10 to engage or retain the hilt portion in its nested position, thus preventing dislocation of the applicator parts during shipment.
- the lid may be taper-fitted with the sides of base member 10 to prevent contamination of the applicator and/or antigens.
- the lid and base may be spot-fused to prevent disassembly prior to use.
- the enclosure formed by the base and lid may be pre-sterilized or, advantageously, made of a material when using ethylene oxide/freon gas for post-assembly sterilization.
- the entire testing kit may be inserted in an envelope having a gas-permeable window.
- the applicator prong or skin-piercing portion of the injection unit may be made from several materials, preferably metal and hard plastics.
- Polished surgical steel cannulae are the prong members found to be advantageous from the standpoint of quality and reproducibility.
- the standard hypodermic needle or cannula of polished steel, having a bevel angle of 12.5°, provides a sharp point which can easily be inserted to the desired skin depth.
- a standard cannula of 15 to 25 guage can be employed, depending upon the desired carrying capacity of the base structure and prong size. For a wide variety of biological substances, a standard 20 guage cannula can provide the dual functions of the prong member.
- the diluent or fluid carrier of the biologicals is often a hydrophilic compound ' or mixture of chemicals which possesses a high surface tension with respect to the prong.
- a capill ry-forming structure permits relatively large amounts of the liquid biological substances and carriers to adhere to the prong.
- a 20 gauge steel needle has been found to retain about 1.8 milligrams of antigen-diluent mixture after dipping.
- the amount of fluid varies according to the particular test composition and prong type, amounts from a few tenths of a milliliter to a few microliters may be feasible.
- a loading of about 0.001 to 0.1 ml is preferred.
- Liquid pickup from the polypropylene type base would ordinarily be in the desired range if a fractional milliliter of liquid extract or chemical mixture is contained in the well. It is understood that a controlled amount of solid or semi-dried biological can be obtained by employing more or less diluent to adjust the active component of the mixture. A relatively large amount of antigen can be picked up
- the amounts of antigen components can be as set forth herein or some other standard may be established for manufacturing convenience or medical purposes.
- Plastic molding compositions such as nylons, polyalkenes, polycarbonates, acrylics, etc. can be employed in making the injection units, bases, covers, etc. Provided an effective point can be cast or molded from plastics, the entire system may be fabricated from one or more synthetic resins. In the preferred embodiments, metal prongs and thermoplastic resin, such as polypropylene, are used.
- the flat base of the applicator may be two-tiered with a central smaller portion adjacent to the cannula and a larger portion near the handle. This type of base disguises the needle puncture and serves as a stop to control depth of penetration of the point of the test prong. This feature makes the needle puncture virtually painless and insures repetitive, standardized penetration of the skin to the desired depth.
- An alternative design is a completely flat hilt.
- hypodermic needle point i.e., sharp, relatively atraumatic skin puncture
- advantages are the utilization of the inner bore of the needle, in the area of the cutting point or bevel, as an inherent capillary trough or liquid reservoir for antigen application.
- the needle point may project from the circular base anywhere from 0.5 to 3.0mm or more, with 2.25mm being optimum for most applicators.
- the injection unit permits the length of needle point projection to be varied without changing the cavity mold used in manu acture.
- the preferred injection unit of Fig. 2 is made of a molded polypropylene plastic.
- the cylindrical handle is hollow with a wall about 1.6mm thick.
- the elongated tubular shape (about 17.5 x 9.5mm diameter) permits easy grasping.
- the two-tier circular hilt is about 2mm thick at the inner circle (8.25 mm) and about 1.5 mm thick for the outer (15.25mm).
- the cannula point and shaft pierce the center of the base, which is molded with a diameter slightly less than the cannula to provide means for holding the cannula in a fixed position by radial gripping force.
- the cannula shaft is additionally supported by a sleeve or cylindrical upward extension of the base for a distance of about 6mm into the hollow core handle.
- the top of the handle is open to allow insertion of the cannula there through and to retain the capillary action.
- FIG. 5 An all-plastic alternative embodiment is shown in Fig. 5, an enlarged cross-sectional view showing the flat plate or hilt portion 23A having a hard prong portion 30A extending downwardly therefrom.
- the prong comprises a skin-piercing point 32A and a reservoir-forming open portion 34A, which is shown as an eyelet having an open area to receive liquid and hold it prior to application.
- the prong portion may have an overall length of 2-4mm. If sufficient liquid holding capacity is achieved by the prong configura ⁇ tion, the eyelet may be omitted.
- the preferred testing method employing the new applicators involves a manual se ⁇ uence in which the individual injections are spaced, at least about 2 cm apart on the skin
- the invention may be adapted or modified to permit simultaneous pickup and application of the entire multi-unit assembly. This can be accomplished by a suitable manipulator device adapted to receive and hold the handle portion of the individual injection units in spaced relationship.
- a suitable manipulator device adapted to receive and hold the handle portion of the individual injection units in spaced relationship.
- FIG. 6 shows a vertical cross-section of a molded receptacle 110 adapted to receive a standard antigen applicator 20.
- the circular applicator disc portion 22 for this configuration is closely mated to the periphery of the base receptacle, thereby forming a seal and resiliently holding the applicator or injection unit with sufficient firmness to prevent separation during handling.
- the base portion shown comprises a concentric depression 112, annular ridge 113 and central well 114.
- a measured quantity of liquid antigen is placed into the center well and the injected unit is inserted into the depression with the cannula point extending into the well.
- a small vent hole 116 located between the annular ridge 113 and the periphery of the depression 112 permits air or other gas to be evacuated as the injection unit 20 is urged into the depression 112. By venting the trapped gas, no excessive pressure is permitted to build in the well 114, which might force an uncontrolled amount of antigen upwardly through the cannula.
- the hilt portion 22 of the applicator is seated against the annular ridge 113, . forming an effective liquid seal.
- the configuration retains a normal capillary loading of the desired amount of antigen at the lower extremity of the cannula. Pressure equalization avoids forcing excess liquid up the cannula during assembly and facilitates quality control of the device. Antigen amounts beyond the normal capillary filling might result in lack of standardization for the intracutaneous deposit.
- the annular ridge 113 may be in the form of a concentric circle on the like; however, any desired shape may be employed.
- the raised surface of this annulus should be sufficiently uniform to provide for liquid containment, when acting in conjunction with the opposed lower hilt surface of the applicator. It is understood that various interlocking surfaces may be employed to effect this sealing function. During assembly, excess liquid that spills outwardly from the well through the sealed annulus may be retained in the outer chamber of the base depression.
- vent hold 116 is shown in a preferred embodiment passing through the base depression outside the annular ridge 113, the chamber may be vented through a hole in the hilt portion 22 of the injection unit or in the base area between the well 114 and annular ridge 113.
- the base may be molded of impact polystyrene advantageously, and the lid may be of the same or different material.
- the number of wells for the base, and their geometric arrangement, can be adapted for several types of test kits. Ordinarily, about 8 to 11 units will be required to provide optimum allergy screening capacity. If the injection device is employed for other biologicals, such as immunogens, a different base arrangement may be adapted.
- the preferred allergy screening and/or diagnostic method for using the applicator kit includes placing common antigens into groups of closely-related com ⁇ ponents for simplicity of testing.
- inhalant or aeroallergens are divided into seven or eight groups depending on the antigens found in a particular geographical location.
- Food antigens may also be divided into groupings.
- antigens are then applied by the individual injection units to the volar surface of the forearm along with controls of the particular diluent used and one of histamine.
- the purpose of using a control consisting essentially of the diluent (devoid of biologically active matter) is to insure against false positive reactions caused by sensitivity to the diluent itself or der ographia.
- the purpose of using a histamine control is to guard against false negative responses brought about by the patient having taken or having had administered a drug having antihistaminic properties within the previous twenty-four to forty-eight hour period (diminished host response).
- inhalant antigens include the following: trees, molds, grasses, ragweed, weeds, Bermuda, dust, and epidermals (dander, animal hair, feathers, etc.). Different and new groupings may be employed, as local conditions determine, and geographical breakdown of the United States into nine territories for the purpose of antigen grouping has been established.
- Food antigens have been classified into nine common fa iliies: whole cow's milk; whole egg; legumes (peas, peanuts and all beans including soybean); chocolate; grains (wheat, rye, barley and corn); citrus fruits (orange, grapefruit and lemon); potato family (including green peppers, tomatoes, and potatoes); seafood and fish family; and cucumber family (cucumber, cantaloupe and watermelon).
- the antigen may be applied to the applicator tip in either an aqueous form or a glycerin-saline base,
- the aqueous form consists of methyl paraben 0.5% and propylparaben 0.05% in N. saline solution.
- the aqueous antigen can be concentrated on the applicator prong by packaging the units with silica gel or other dessicant.
- the antigen may be dehydrated by controlled temperature dehydration; i.e., less than 39° C, to prevent denaturing the biologicals.
- This dehydrated form of antigen has adequate shelf-life and becomes biologically active when introduced into the skin.
- the glycerin-saline base antigen (equal volumes of glycerin and N. saline) is simply applied to the tip of the applicator by dipping and left in a nondehydrated state for shipment and use.
- Antigens may be applied in mass production by filling the corresponding well of the base, in which the applicator is housed for shipment. The advantage of this method is less labor and expense of production as well as adequate stability and shelf-life.
- the cannula is electrically conductive, certain biological substances can be deposited electrophoretically from a suitable aqueous or nonaqueous dispersion by biasing the cannula with a direct current potential.
- the preferred concentration is 50 grams/liter (g/1).
- the preferred concentration is lOOg/l. These concentrations will render 20,000 protein nitrogen units per c.c. Because of the 50% glycerin, the shelf-life of the antigen is several years. Individual kits are assembled and gas sterilized with a gaseous mixture of 88% ethylene oxide and 12% Freon.
- each kit will have two controls, one control consisting of histamine phosphate (0.55g/l).
- the different antigen groups and controls may have a different colored applicator for coding.
- the base may have recessed depressions of particular individual shape to accommodate a distinctive hilt shape for each biological or control substance.
- the flat plate may be in a circular, oval, square, triangular, octagonal or other desired shape to prevent confusion.
- the invention is a new diagnostic and diagnostic screening technique for use in inhalant allergy (aeroallergens) and food allergy. It incorporates the use of a unique antigen applicator. Any physician or supervised staff can, by use of the test kit, diagnose and/or screen a patient for inhalant or food allergy. This is accomplished simply, inexpensively, accurately and virtually painlessly. In addition, this technique is inherently safer than many current intradermal farnesy testing methods.
- a patient or subject does not give positive reactions to the initial testing, there is probably no significant aeroallergen or food sensitivity. This obviates the need of subjecting the patient to needless, costly and time-consuming further testing. If on the other hand, the patient demonstrates a positive reaction to multiple-allergen testing, further delineation of the offending antigen can then be conducted via either scratch testing, specific intradermal or the serial dilution technique. The practitioner may treat the patient in a known manner by injecting the multiple-antigen mixture to which a positive reaction has been observed. Likewise, an individual component of a positive antigen mixture may be employed for hyposensitization after identification of the antigen by delineating the mixture.
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Abstract
A skin-testing system for in vivo intracutaneous use which comprises a novel injection unit and multiple applicator means, each of the units carrying biological or chemical substances for skin-testing, at least one of the units carrying a plurality of different antigens in admixture. Test substances are deposited intracutaneously by piercing the skin with each injection to predetermined depth; and the pierced skin is observed for response to the various substances and dermographia. The preferred applicator means comprises points carrying groups of admixed allergens selected from tree allergens, mold allergens, grass allergens, ragweed allergens, weed allergens, dust, epidermals and foods together with histamine control, and diluent control. Each of the injection units (20) includes a handle portion (25), hilt portion (22) and a scarifier portion (32) having means for carrying testing substances. A base member (10, 110) is provided with a plurality of recessed depressions (12, 112) adapted to receive and hold the injection units individually, with the scarifier portion or needle-like prong being received by a well portion (14, 114) containing antigens or the like. In a preferred embodiment each of the depressions is provided with vent means (116) for permitting gas escape.
Description
Description
Allergy Testing System
The present invention relates to skin testing with biological substances. In particular, it relates to medical methods and devices for allergy detection, including intracutaneous injuction of biologicals,' such as aeroallergens, food allergens, and other chemical substances.
Diagnosis of allergies in the past has depended upon a number of techniques for introducing various biological substances to the epidermis or der is. In a widely-accepted testing method for inhalant allergy - the scratch test - various allergenic sub¬ stances are applied by abrading or cutting the epidermal layer and contacting a liquid allergenic extract or the like with the exposed skin tissue. These test areas are often on the back of a human patient, who may be subject to many painful tests. The superficial scratches or abrasions produce a less severe reaction than dermal injection. If no response or weak responses are obtained in the scratch tests, less concentrated allergens may be applied to the upper extremities of the patient intradermaliy with a small bore needle and syringe. Reactions to these latter tests may be dramatic and even require emergency measures due to the severity of the reaction.
In another allergy testing method, a series of
intradermal injections is administered by the laborious needle and syringe procedure, employing allergens in various dilutions for safety and therapeutic reasons. This serial dilution technique requires a highly skilled technician and is tedious, expensive, and often painful to the patient. However, these in vivo allergy testing methods are the primary test methods employed by allergists and otolaryngolo- gists currently. In vitro test methods, such as radioi munoassays, require considerable laboratory equipment and are not generally accepted for screening patients on a preliminary basis.
In addition to the airborne allergens, food allergens have been tested by skin response and are of interest to many workers in the medical field..
Besides the epidermal scratch and intradermal allergy testing methods, scarifiers have found use in applying other biological substances. For instance, vaccinations may be effected with such devices. Antigens have been applied intradermally for the Heaf multiple puncture tuberculin test.
Various attempts have been made to simplify the testing of allergies to reduce the amount of time necessary for effecting application of allergenic substances. Multiple skin tests have been administered simultaneously by applying a plurality of spaced scarifiers or puncture heads dipped in liquid antigens; however, this method has not proven entirely satisfactory due to the difficulty of locating a number of effective test sites in predetermined geometric pattern. Care must be taken in administering
O
intradermal antigens not to inject the biological substance into a blood vessel, and this limitation on the practical use of spaced multipoint applicators has discouraged its adoption for intradermal testing. The present invention provides a system for allergy testing wherein common antigens are incorporated in a plurality of injector units adapted for intracutaneous use. The individual injector units are intended to be supplied as part of a multiple-allergen screening and/or diagnostic kit.
A new skin test device for intracutaneous use has been devised. This device is an applicator or injection unit having a hilt or flat plate portion and a hollow rigid handle portion attached to the plate portion on one side thereof and adapted for grasping the device. In order to pierce the skin, a hollow metal cannula scarifier element is mounted on the flat plate, extending outwardly from the flat plate opposite the handle portion a predetermined length for intradermal injection. The cannula has a sharp skin-piercing point at its lower extremity and a shaft portion extending upwardly through the flat plate into said hollow handle portion. This configuration permits the device to be loaded with a predetermined amount of fluent skin testing substance, which may be applied to the point by dipping and distributed into the hollow scarifier by capillary action.
The flat plate portion and handle portion may be integrally molded of thermoplastic resin, such as polypropylene. In the preferred embodiment of the skin test device, the handle portion comprises an
elongated cylindrical tube having an open top end, and the flat plate portion has a sleeve projecting upwardly into the hollow handle portion for holding the scarifier element firmly with a predetermined prong length exposed below the hilt.
An allergy testing kit for multiple allergen screening may be assembled with a number of these applicators or injection units. A base member comprising a plurality of recessed depressions, each having a well portion adapted to receive a needle-like prong, is provided with the kit. A corresponding number of intracutaneous injection units adapted for being held in the recessed depression of the base member is provided, each comprising a hilt portion adapted for insertion into a complementary recessed depression of base member. A downwardly extending skin test prong portion is adapted for insertion into the corresponding well. The upwardly extending handle portion can be grasped manually for applying the injection units sequentially. In the test kit at least one of the prongs is loaded with a mixture of biologically active allergens, at least one of the prongs is loaded with a histamine control substance, and at lease one of the prongs is loaded with a diluent devoid of biologically active substance.
The assembled kit may include a sealed package of ethylene-oxide-permeable material for containing the base member and injection units, permitting sterilization after assembly. Advantageously, the test prongs comprise a hollow cannula or hypodermic needle extending from the hilt into the base well
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about 0.5 to 3 mm, and the handle portion is hollow to receive an upper shaft portion of the cannula. This permits capillary loading of the prongs by dipping the prong into a liquid. The invention will be further explained in the following description and in the drawing, wherein: FIG. 1 is a perspective view of the novel applicator system, showing the base and an injection unit; FIG. 2 is a vertical cross-section view of an injection unit;
FIG. 3 is a schematic view of the injection unit during use;
FIG. 4 is a vertical cross-section view of the packaged base containing an injection unit;
FIG. 5 is a partial cross-section view of an alternative embodiment; and
FIG. 6 is a cross-section view of a preferred embodiment of the invention showing a modified base member with vent- means.
In the following description, all measurements and dimensions are given in metric units and parts by- weight unless otherwise stated.
Referring to Fig. 1, a base member 10 in the form of a stable flat tray is provided with a plurality of recessed depressions 12 adapted to receive individually removable applicators or injection units 20. The depressions are aligned in one or more rows for ease of identification and to facilitate use cf the individual applicators. An enlarged sectional view of a single injection unit 20 is depicted in Fig.
2. In this preferred embodiment, a metal cannula is held firmly in the hilt portion 22 of the injection unit. The hilt portion comprises a flat plate, with a two-tier configuration 22, 23. The handle portion 25 shown as an elongated cylindrical tube, may have an opening at its top end or elsewhere to permit gas access to the interior or the injection unit. This aids in manufacture, liquid loading and sterilization of the fabricated applicator system. To provide a firm gripping force on the cannula 30, the flat plate or hilt portion 22 of the injection unit has a sleeve 28 projecting upward into the hollow handle portion. This prevents slippage during use of the cannula 30 as a scarifier, with a predetermined length exposed below the flat plate or hilt 22, 23.
During loading of liquid biologicals or other fluid materials, the cannula may be dipped into the fluid, with the skin-piercing point 32 being received into a well to prevent damaging the point. A hollow portion 34 provides a liquid reservoir on the cannula scarifier element 30, 32.
During use of skin testing, the injection unit 20 is removed manually from the base and inserted into the skin, as shown in Fig. 3. The hollow metal scarifier element 30 pierces the epidermal layer 40 and extends there through into the dermis 42, where the substance carried on the scarifier prong is deposited intracutaneously. Ordinarily, -the injection unit is withdrawn immediately after injecting the test substance. The base member 10 may be packaged as part of a testing kit, as shown in Fig. 4. The base is
Λ
provided with a plurality of circular depressions 12 into which the hilt portion of injection unit 20 is inserted. The bottom of this recessed portion is tapered downwardly to a depth of about 3mm, premitting the lower prong tip 32 to be accommodated within a well 14, which may be conoidal in shape. Prior to inserting the injection unit, a measured quantity of the particular biological substance or diluent is placed in the bottom of the well, 14. In order to protect the testing kit after manufacture and sterilization, a lid 18 is placed over the base member 10, preventing the individual injection units from becoming loose. As an extra precaution, a projecting segment 16 can be molded onto the base 10 to engage or retain the hilt portion in its nested position, thus preventing dislocation of the applicator parts during shipment. The lid may be taper-fitted with the sides of base member 10 to prevent contamination of the applicator and/or antigens. The lid and base may be spot-fused to prevent disassembly prior to use. The enclosure formed by the base and lid may be pre-sterilized or, advantageously, made of a material when using ethylene oxide/freon gas for post-assembly sterilization. Alternatively, the entire testing kit may be inserted in an envelope having a gas-permeable window.
The applicator prong or skin-piercing portion of the injection unit may be made from several materials, preferably metal and hard plastics. Polished surgical steel cannulae are the prong members found to be advantageous from the standpoint of quality and
reproducibility. The standard hypodermic needle or cannula of polished steel, having a bevel angle of 12.5°, provides a sharp point which can easily be inserted to the desired skin depth. A standard cannula of 15 to 25 guage can be employed, depending upon the desired carrying capacity of the base structure and prong size. For a wide variety of biological substances, a standard 20 guage cannula can provide the dual functions of the prong member. The diluent or fluid carrier of the biologicals is often a hydrophilic compound' or mixture of chemicals which possesses a high surface tension with respect to the prong. A capill ry-forming structure permits relatively large amounts of the liquid biological substances and carriers to adhere to the prong. Typically, - a 20 gauge steel needle has been found to retain about 1.8 milligrams of antigen-diluent mixture after dipping.
While the amount of fluid varies according to the particular test composition and prong type, amounts from a few tenths of a milliliter to a few microliters may be feasible. For allergenic extracts of the kinds described herein, a loading of about 0.001 to 0.1 ml is preferred. Liquid pickup from the polypropylene type base would ordinarily be in the desired range if a fractional milliliter of liquid extract or chemical mixture is contained in the well. It is understood that a controlled amount of solid or semi-dried biological can be obtained by employing more or less diluent to adjust the active component of the mixture. A relatively large amount of antigen can be picked up
. W
by surface phenomena when less diluent is present. For purposes of product uniformity, the amounts of antigen components can be as set forth herein or some other standard may be established for manufacturing convenience or medical purposes.
Plastic molding compositions, such as nylons, polyalkenes, polycarbonates, acrylics, etc. can be employed in making the injection units, bases, covers, etc. Provided an effective point can be cast or molded from plastics, the entire system may be fabricated from one or more synthetic resins. In the preferred embodiments, metal prongs and thermoplastic resin, such as polypropylene, are used.
The flat base of the applicator may be two-tiered with a central smaller portion adjacent to the cannula and a larger portion near the handle. This type of base disguises the needle puncture and serves as a stop to control depth of penetration of the point of the test prong. This feature makes the needle puncture virtually painless and insures repetitive, standardized penetration of the skin to the desired depth. An alternative design is a completely flat hilt.
Aside ' from the obvious advantage of the hypodermic needle point; i.e., sharp, relatively atraumatic skin puncture, there are other advantages. These advantages are the utilization of the inner bore of the needle, in the area of the cutting point or bevel, as an inherent capillary trough or liquid reservoir for antigen application.
The needle point may project from the circular base anywhere from 0.5 to 3.0mm or more, with 2.25mm being optimum for most applicators. The injection unit permits the length of needle point projection to be varied without changing the cavity mold used in manu acture.
The preferred injection unit of Fig. 2 is made of a molded polypropylene plastic. The cylindrical handle is hollow with a wall about 1.6mm thick. The elongated tubular shape (about 17.5 x 9.5mm diameter) permits easy grasping. The two-tier circular hilt is about 2mm thick at the inner circle (8.25 mm) and about 1.5 mm thick for the outer (15.25mm). The cannula point and shaft pierce the center of the base, which is molded with a diameter slightly less than the cannula to provide means for holding the cannula in a fixed position by radial gripping force. The cannula shaft is additionally supported by a sleeve or cylindrical upward extension of the base for a distance of about 6mm into the hollow core handle. The top of the handle is open to allow insertion of the cannula there through and to retain the capillary action.
An all-plastic alternative embodiment is shown in Fig. 5, an enlarged cross-sectional view showing the flat plate or hilt portion 23A having a hard prong portion 30A extending downwardly therefrom. The prong comprises a skin-piercing point 32A and a reservoir-forming open portion 34A, which is shown as an eyelet having an open area to receive liquid and hold it prior to application. The prong portion may
have an overall length of 2-4mm. If sufficient liquid holding capacity is achieved by the prong configura¬ tion, the eyelet may be omitted.
While the preferred testing method employing the new applicators involves a manual seσuence in which the individual injections are spaced, at least about 2 cm apart on the skin, it is understood that the invention may be adapted or modified to permit simultaneous pickup and application of the entire multi-unit assembly. This can be accomplished by a suitable manipulator device adapted to receive and hold the handle portion of the individual injection units in spaced relationship. However, the afore¬ mentioned difficulties in avoiding blood vessels must be taken into account for any such multi-point application.
Another embodiment of the base is depicted in Fig. 6, which shows a vertical cross-section of a molded receptacle 110 adapted to receive a standard antigen applicator 20. The circular applicator disc portion 22 for this configuration is closely mated to the periphery of the base receptacle, thereby forming a seal and resiliently holding the applicator or injection unit with sufficient firmness to prevent separation during handling.
The base portion shown comprises a concentric depression 112, annular ridge 113 and central well 114. A measured quantity of liquid antigen is placed into the center well and the injected unit is inserted into the depression with the cannula point extending into the well. A small vent hole 116 located between
the annular ridge 113 and the periphery of the depression 112 permits air or other gas to be evacuated as the injection unit 20 is urged into the depression 112. By venting the trapped gas, no excessive pressure is permitted to build in the well 114, which might force an uncontrolled amount of antigen upwardly through the cannula. The hilt portion 22 of the applicator is seated against the annular ridge 113, . forming an effective liquid seal. The configuration retains a normal capillary loading of the desired amount of antigen at the lower extremity of the cannula. Pressure equalization avoids forcing excess liquid up the cannula during assembly and facilitates quality control of the device. Antigen amounts beyond the normal capillary filling might result in lack of standardization for the intracutaneous deposit.
The annular ridge 113 may be in the form of a concentric circle on the like; however, any desired shape may be employed. The raised surface of this annulus should be sufficiently uniform to provide for liquid containment, when acting in conjunction with the opposed lower hilt surface of the applicator. It is understood that various interlocking surfaces may be employed to effect this sealing function. During assembly, excess liquid that spills outwardly from the well through the sealed annulus may be retained in the outer chamber of the base depression.
While the vent hold 116 is shown in a preferred embodiment passing through the base depression outside the annular ridge 113, the chamber may be vented
through a hole in the hilt portion 22 of the injection unit or in the base area between the well 114 and annular ridge 113. In the embodiment of Fig. 6, the base may be molded of impact polystyrene advantageously, and the lid may be of the same or different material.
The number of wells for the base, and their geometric arrangement, can be adapted for several types of test kits. Ordinarily, about 8 to 11 units will be required to provide optimum allergy screening capacity. If the injection device is employed for other biologicals, such as immunogens, a different base arrangement may be adapted.
The preferred allergy screening and/or diagnostic method for using the applicator kit includes placing common antigens into groups of closely-related com¬ ponents for simplicity of testing. Typically, inhalant or aeroallergens are divided into seven or eight groups depending on the antigens found in a particular geographical location. Food antigens may also be divided into groupings.
These antigens are then applied by the individual injection units to the volar surface of the forearm along with controls of the particular diluent used and one of histamine. The purpose of using a control consisting essentially of the diluent (devoid of biologically active matter) is to insure against false positive reactions caused by sensitivity to the diluent itself or der ographia. The purpose of using a histamine control is to guard against false negative responses brought about by the patient having taken or
having had administered a drug having antihistaminic properties within the previous twenty-four to forty-eight hour period (diminished host response). The preferred groupings of inhalant antigens include the following: trees, molds, grasses, ragweed, weeds, Bermuda, dust, and epidermals (dander, animal hair, feathers, etc.). Different and new groupings may be employed, as local conditions determine, and geographical breakdown of the United States into nine territories for the purpose of antigen grouping has been established.
Because of the large number of trees to be tested in some areas, there can be two tree pollen applicators per kit. One will be the major pollinating trees and the other the minor pollinating trees.
Food antigens have been classified into nine common fa iliies: whole cow's milk; whole egg; legumes (peas, peanuts and all beans including soybean); chocolate; grains (wheat, rye, barley and corn); citrus fruits (orange, grapefruit and lemon); potato family (including green peppers, tomatoes, and potatoes); seafood and fish family; and cucumber family (cucumber, cantaloupe and watermelon). The antigen may be applied to the applicator tip in either an aqueous form or a glycerin-saline base, The aqueous form consists of methyl paraben 0.5% and propylparaben 0.05% in N. saline solution. The aqueous antigen can be concentrated on the applicator prong by packaging the units with silica gel or other dessicant.
1f
The antigen may be dehydrated by controlled temperature dehydration; i.e., less than 39° C, to prevent denaturing the biologicals. This dehydrated form of antigen has adequate shelf-life and becomes biologically active when introduced into the skin. The glycerin-saline base antigen (equal volumes of glycerin and N. saline) is simply applied to the tip of the applicator by dipping and left in a nondehydrated state for shipment and use. Antigens may be applied in mass production by filling the corresponding well of the base, in which the applicator is housed for shipment. The advantage of this method is less labor and expense of production as well as adequate stability and shelf-life. Since the cannula is electrically conductive, certain biological substances can be deposited electrophoretically from a suitable aqueous or nonaqueous dispersion by biasing the cannula with a direct current potential. For trees, weeds, and grasses, the preferred concentration is 50 grams/liter (g/1). For mold, epidermals and house dust, the preferred concentration is lOOg/l. These concentrations will render 20,000 protein nitrogen units per c.c. Because of the 50% glycerin, the shelf-life of the antigen is several years. Individual kits are assembled and gas sterilized with a gaseous mixture of 88% ethylene oxide and 12% Freon. Preferably each kit will have two controls, one control consisting of histamine phosphate (0.55g/l). The other control of a blank control consisting of glycerin and saline.
It is advantageous to provide distinctive markings on each injection unit. The different antigen groups and controls may have a different colored applicator for coding. The base may have recessed depressions of particular individual shape to accommodate a distinctive hilt shape for each biological or control substance. For instance, the flat plate may be in a circular, oval, square, triangular, octagonal or other desired shape to prevent confusion.
The invention is a new diagnostic and diagnostic screening technique for use in inhalant allergy (aeroallergens) and food allergy. It incorporates the use of a unique antigen applicator. Any physician or supervised staff can, by use of the test kit, diagnose and/or screen a patient for inhalant or food allergy. This is accomplished simply, inexpensively, accurately and virtually painlessly. In addition, this technique is inherently safer than many current intradermal alergy testing methods.
If a patient or subject does not give positive reactions to the initial testing, there is probably no significant aeroallergen or food sensitivity. This obviates the need of subjecting the patient to needless, costly and time-consuming further testing. If on the other hand, the patient demonstrates a positive reaction to multiple-allergen testing, further delineation of the offending antigen can then be conducted via either scratch testing, specific intradermal or the serial dilution technique. The practitioner may treat the patient in a known manner
by injecting the multiple-antigen mixture to which a positive reaction has been observed. Likewise, an individual component of a positive antigen mixture may be employed for hyposensitization after identification of the antigen by delineating the mixture. In addition to the benefits of reduced cost in time and money, as well as discomfort from numerous allergy tests, the chances of untoward reaction are reduced numerically by use of the present system. While the invention has been described by particular example, there is no intent to limit the inventive concept except as set forth in the following claims.
Claims
1. An allergy testing kit for multiple allergen screening comprising: a base member comprising a plurality of recessed depressions each having a well portion adapted to receive a needle-like prong; a plurality of intracutaneous injection units adapted for being held in the recessed
10 depressions of said base member, each of said injection units comprising a hilt portion adapted for insertion into the recessed depression of base member, an upwardly extending handle portion and a
15 downwardly extending skin test prong portion adapted for insertion into a corresponding well; at least one of said prongs being loaded
with biologically active allergen; and at least one of said prongs being loaded with a histamine control substance; and at least one of said prongs being loaded with a diluent devoid of biologically active substance.
2. The testing kit of claim 1 wherein each prong comprises a hollow metal cannula extending from the hilt into the wells about 0.5 to 3mm, and wherein the handle portion of each injection unit is hollow to receive an upper portion of said cannula, thereby permitting capillary loading of the prongs by dipping the prong into a liquid.
3. The testing kit of claim 2 as herein said base member depressions are provided with vent means for gas escape.
4. The testing kit of claim 3 wherein each of said depressions has annular ridge means disposed within said depression surrounding said well portion, and wherein said vent means comprises at least one hole communicating with that portion of said depression outside said annular ridge means.
5. A skin test device for intracutaneous use comprising: a flat plate portion; a hollow rigid handle portion attached to the plate portion on one side thereof and adapted for manually grasping the device; and
OMPI a hollow metal cannula scarifier element mounted on said flat plate and extending outwardly from said flat plate opposite said handle portion a predetermined length for intracutaneous injection, said scarifier having a sharp skin-piercing hollow point at its lower extremity and an upper shaft portion extending upwardly through said flat plate into said hollow handle portion; whereby said device may be loaded with a predetermined amount of fluent skin testing substance applied to said point by dipping and distributed into the hollow scarifier by capillary action.
6. The skin test device of claim 4 wherein said flat plate portion and handle portion are integrally molded.
7. The device of claim 6 wherein the plate and handle portion consist essentially of thermoplastic resin.
8. The skin test device of claim 7 wherein the thermoplastic resin comprises polypropylene.
9. The skin test device of claim 5 wherein the handle portion comprises an elongated cylindrical- tube having an open top end, and wherein the flat plate portion has a sleeve projecting upwardly into said hollow handle portion for holding the shaft portion of scarifier element firmly with the predetermined length exposed below said flat plate portion.
10. A skin testing method for in vivo intracu- taneous use which comprises the steps of: providing applicator means comprising a plurality of individual injection units, each of said injection units comprising a handle portion, a hilt portion and a scarifier portion comprising a skin piercing intradermal point and having means for carrying testing substances, each of said units carrying biological or chemical substances for skin testing, at least one injection unit of said applicator means carrying a plurality of different antigens in admixture; depositing said substances intracutaneously by piercing the .skin with each unit to predetermined depth; and observing the pierced skin for response to said substances and demographia.
11. The method of claim 10 wherein the applicator means comprises at least one injection unit loaded with a predetermined effective amount of admixed allergens selected from tree allergens, mold allergens, grass allergens, ragweed allergens, epidermals, dust and weed allergens; and wherein said applicator means further comprises histamine control substances and diluent control substances.
Applications Claiming Priority (3)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| US939442 | 1978-09-05 | ||
| US05/939,442 US4205689A (en) | 1978-09-05 | 1978-09-05 | Allergy testing system |
| US06/041,957 US4222392A (en) | 1979-05-23 | 1979-05-23 | Allergy testing device with vented base |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| WO1980000531A1 true WO1980000531A1 (en) | 1980-04-03 |
Family
ID=26718735
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| PCT/US1979/000553 WO1980000531A1 (en) | 1978-09-05 | 1979-07-30 | Allergy testing system |
Country Status (2)
| Country | Link |
|---|---|
| EP (1) | EP0016198A1 (en) |
| WO (1) | WO1980000531A1 (en) |
Cited By (3)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| EP0224225A1 (en) * | 1985-11-28 | 1987-06-03 | BEHRINGWERKE Aktiengesellschaft | Device for the interdermatological application of testing matter and vaccines |
| WO1994027147A1 (en) * | 1993-05-14 | 1994-11-24 | Universiteit Utrecht | A method of screening food products for food allergenicity |
| FR2748647A1 (en) * | 1996-05-20 | 1997-11-21 | Stallergenes Sa | Scarifying implement for allergy tests |
Families Citing this family (1)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| GB0420256D0 (en) | 2004-09-13 | 2004-10-13 | Cassells John M | Method and apparatus for sampling and analysis of fluids |
Citations (9)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US2522309A (en) * | 1948-12-01 | 1950-09-12 | Frank A Simon | Allergy testing instrument |
| US2841138A (en) * | 1957-03-11 | 1958-07-01 | Ernest S V Laub | Allergy testing device |
| US3034507A (en) * | 1960-05-10 | 1962-05-15 | American Cyanamid Co | Intracutaneous injection device |
| US3123212A (en) * | 1964-03-03 | Multiple disposable intracutaneous injector package | ||
| US3289670A (en) * | 1964-03-09 | 1966-12-06 | Milo Bundy Corp | Device for abrading and applying biologicals to the skin of a patient |
| US3444989A (en) * | 1967-01-05 | 1969-05-20 | Behringwerke Ag | Casing for devices for intradermal application |
| US3556080A (en) * | 1968-04-08 | 1971-01-19 | Lincoln Lab Inc | Skin allergy testing device |
| US3596660A (en) * | 1969-05-12 | 1971-08-03 | Illinois Tool Works | Injection device |
| US3688764A (en) * | 1970-08-20 | 1972-09-05 | Bard Hamilton Co Inc | Intracutaneous injection system |
-
1979
- 1979-07-30 WO PCT/US1979/000553 patent/WO1980000531A1/en unknown
-
1980
- 1980-04-08 EP EP19790901023 patent/EP0016198A1/en not_active Withdrawn
Patent Citations (9)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US3123212A (en) * | 1964-03-03 | Multiple disposable intracutaneous injector package | ||
| US2522309A (en) * | 1948-12-01 | 1950-09-12 | Frank A Simon | Allergy testing instrument |
| US2841138A (en) * | 1957-03-11 | 1958-07-01 | Ernest S V Laub | Allergy testing device |
| US3034507A (en) * | 1960-05-10 | 1962-05-15 | American Cyanamid Co | Intracutaneous injection device |
| US3289670A (en) * | 1964-03-09 | 1966-12-06 | Milo Bundy Corp | Device for abrading and applying biologicals to the skin of a patient |
| US3444989A (en) * | 1967-01-05 | 1969-05-20 | Behringwerke Ag | Casing for devices for intradermal application |
| US3556080A (en) * | 1968-04-08 | 1971-01-19 | Lincoln Lab Inc | Skin allergy testing device |
| US3596660A (en) * | 1969-05-12 | 1971-08-03 | Illinois Tool Works | Injection device |
| US3688764A (en) * | 1970-08-20 | 1972-09-05 | Bard Hamilton Co Inc | Intracutaneous injection system |
Cited By (4)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| EP0224225A1 (en) * | 1985-11-28 | 1987-06-03 | BEHRINGWERKE Aktiengesellschaft | Device for the interdermatological application of testing matter and vaccines |
| WO1994027147A1 (en) * | 1993-05-14 | 1994-11-24 | Universiteit Utrecht | A method of screening food products for food allergenicity |
| NL9300846A (en) * | 1993-05-14 | 1994-12-01 | Friesland Frico Domo Coop | Method for screening food products for food allergy. |
| FR2748647A1 (en) * | 1996-05-20 | 1997-11-21 | Stallergenes Sa | Scarifying implement for allergy tests |
Also Published As
| Publication number | Publication date |
|---|---|
| EP0016198A1 (en) | 1980-10-01 |
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