CN212904942U

CN212904942U - Sample detector

Info

Publication number: CN212904942U
Application number: CN202020461477.0U
Authority: CN
Inventors: 洪亮; 周凯军
Original assignee: Hangzhou Biotest Biotech Co Ltd
Current assignee: Hangzhou Biotest Biotech Co Ltd
Priority date: 2020-04-01
Filing date: 2020-04-01
Publication date: 2021-04-06
Anticipated expiration: 2030-04-01

Abstract

The utility model provides a sample detector, which comprises a mixing cavity and a detection cavity, wherein the mixing cavity is filled with detection liquid, a sample can be added into the mixing cavity, after the sample is added, the detection liquid is mixed with the sample, and the sample is dissolved in the detection liquid to obtain mixed liquid; a test element is arranged in the detection cavity and used for detecting whether the mixed solution contains the analyte or not; wherein, be equipped with sealing element between mixing chamber and the detection chamber, a part on the sealing element extends to the detector outside, and sealing element can be promoted. The utility model discloses the occult blood detection of being applied to excrement that can be fine, the base of making through the cup body that opaque material made and transparent material, recycle ultrasonic welding technique and close both as an organic whole, can avoid operating personnel to look directly at and contact excrement in the testing process, can be very audio-visual through observing the test strip in the base simultaneously and obtain the testing result.

Description

Sample detector

Technical Field

The utility model belongs to the technical field of the medical instrument technique and specifically relates to a can be used for sample detector of liquid, solid sample.

Background

In the field of medical biology, the analysis and detection of samples is a whole process, and the analysis and detection of samples is the basis of numerous tests and treatments. The detection of solid sample generally needs to be mixed with detection liquid for reaction, the mixing process of the sample and the detection liquid relates to the problem of solid sample quantification, the operation is more complicated, and in addition, for some samples with pollution properties, operators have the requirements of safety and sanitation and are inconvenient to directly contact.

The excrement is a common solid sample, and excrement occult blood detection can early warn the abnormality of the digestive tract, and when the amount of bleeding in the digestive tract is less, the appearance of the excrement can not be changed abnormally and can not be identified by naked eyes. A plurality of large-scale cohort studies prove that the incidence and mortality of colorectal cancer of people can be obviously reduced by detecting fecal occult blood every year. Fecal occult blood detection is recommended as the colorectal cancer screening technology of the most main population by a plurality of authoritative organizations such as American cancer society, early diagnosis and early treatment projects of colorectal cancer of the national ministry of health of China, and digestive diseases of the Chinese medical society.

In the conventional fecal occult blood detection, a subject needs to take stool for inspection and the professional in a hospital detects the stool. However, because of the high requirements for specimen preservation and transportation in stool collection and examination, people who attend physical examinations in hospitals often choose to ignore or not to examine the stool because of inconvenience. Therefore, in actual population screening and physical examination, the stool sampling and examination rate is low. In a colorectal cancer screening test in the Xuhui area and the Haerbin south sentry area, the excrement submission rate of community residents is less than 40%.

In fact, the colloidal gold immune test paper on the market is very simple to detect the fecal occult blood, is similar to the early pregnancy test paper, and can be completely detected by community residents at home and judge the result by the community residents. But people are reluctant to look directly or touch the stool due to the strong smell of the stool. Secondly, the excrement is solid and needs to be fully dissolved in the detection liquid before the detection of the immune test paper can be carried out. Again, control of stool sample size is difficult. Finally, the detection operation must ensure that the excrement is dissolved in the detection solution and then does not overflow or leak, otherwise, the detection is not suitable for household or non-specialized household detection. At present, no instrument suitable for fecal occult blood self-detection exists in the market, and although some fecal occult blood reagent manufacturers respectively design some excrement collectors, the excrement collectors do not have sampling amount control devices and do not comprise detectors, and all detections are performed under open conditions. Therefore, at present, fecal occult blood is only carried out in a professional medical institution, a professional generally places quantitative fecal into a container with detection liquid for dissolving, then pours the fecal liquid in the container into a small cup or a small hole, then inserts a liquid absorption test strip into the small cup or the small hole for detection, according to the colloidal gold immunochromatography principle, the mixed liquid contacts with the test strip in the kit to run out, a color band appears, and the fecal occult blood is judged to be negative or positive according to the comparison of the color depth of the color band and a standard color card. The fecal liquid is open during detection, the number of times of direct vision of excrement is large, the small cup and the small hole are easy to overturn and overflow and leak the liquid during operation, the operation is carried out by wearing gloves, and the detection devices are not dispersed into a whole set and are inconvenient to carry and transport, so that the existing excrement occult blood cannot be automatically determined by non-professionals.

Disclosure of Invention

An object of the utility model is to provide a sample detector to solve the problem that proposes among the above-mentioned background art.

The utility model aims at the defects of the prior sample detector, and provides a sample collecting detector to solve the technical problems mentioned above, the sample monitor is mainly applied to the detection of substances such as excrement and urine, and the technical proposal adopted by the utility model is a sample detector which comprises a mixing cavity, a detection cavity and a sealing element, wherein, the mixing cavity is filled with detection liquid, the sample can be added into the mixing cavity, after the sample is added, the detection liquid is mixed with the sample, and the sample is dissolved in the detection liquid to obtain mixed liquid;

a test element is arranged in the detection cavity and used for detecting whether the mixed solution contains the analyte or not;

the sealing element comprises at least two operating positions: the sealing element comprises a first working position and a second working position, wherein when the sealing element is in the first working position, the mixing cavity and the detection cavity are in a non-communication state; when the sealing element is in the second working position, the mixing chamber is in a state of communication with the detection chamber.

Further, the sealing member has elasticity.

Furthermore, a groove is arranged on the sealing element, and when the sealing element is located at the second working position, the groove communicates the mixing cavity with the detection cavity.

Further, the sealing element also comprises a third working position, and when the sealing element is in the third working position, the mixing cavity and the detection cavity are in a non-communication state.

Furthermore, the process of changing the sealing element from the first operating position into the second operating position or vice versa is irreversible.

Furthermore, the sealing element comprises a first sealing part, and a first communication hole is formed between the mixing cavity and the detection cavity;

when the sealing element is in the first working position, the first sealing part is positioned in the first communicating hole, and the first sealing part seals the first communicating hole;

when the sealing element is at the second working position, the first sealing part is separated from the first sealing hole, and the mixing cavity is communicated with the detection cavity.

Further, the sealing element also comprises a second sealing position, and when the sealing element is in the third working position, the second sealing position seals the first communication hole.

Furthermore, a second sealing hole communicated with the outside is formed in the detection cavity, and when the sealing element is located at the first working position, the second working position or the third working position, the second sealing part seals the second sealing hole all the time.

Furthermore, the sealing element is provided with a first annular bulge and a second annular bulge, when the sealing element is located at the first working position, the first annular bulge is attached to the inner wall of the mixing cavity, and the second annular bulge is attached to the outer wall of the detection cavity.

Further, a first annular embossment is located on the first sealing location and a second annular embossment is located on the second sealing location.

To sum up, the utility model has the advantages that: the utility model provides a sample detector can be fine be applied to excrement occult blood and detect, through the cup body that opaque material made and the base that transparent material made, recycle ultrasonic welding technique and combine both into an organic whole, can avoid operating personnel to look at directly and contact the excrement in the testing process, can very audio-visually obtain the testing result through observing the test strip in the base simultaneously; the communication relation between the mixing cavity and the detection cavity is controlled by a sealing element, one part of the sealing element is positioned outside the device, in an initial state, the mixing cavity and the detection cavity are in a non-communication state, the sealing element can move into the device by pressing the part of the sealing element positioned outside the device, the mixing cavity and the detection cavity can be in a communication state, the process of pressing the sealing element can be divided into four stages, each stage can be judged by pressing and pressing by hands, and can also be directly observed by a transparent base; the cover body can be quickly combined with the sample cavity cover to keep tight, so that the odor of excrement can be isolated, and the detection process is clean and sanitary; the design of pairing of application of sample hole and sample collector lets the sampling process need not control the volume of gathering, and the application of sample hole can carry out the ration to the sample that gets into the hybrid chamber inside, and unnecessary sample is preserved in the sample intracavity, and is very convenient, and the while sample of staying of sample intracavity makes things convenient for the resident to carry the shit sample to the hospital and carries out the secondary inspection.

Drawings

FIG. 1 is a schematic view of the overall structure of the sample testing device of the present invention;

FIG. 2 is an exploded view of the sample testing device of the present invention;

FIG. 3 is a sectional view of the entire structure of the sample testing device of the present invention;

FIG. 4 is an enlarged partial schematic view of region "A" of FIG. 3 (first stage);

FIG. 5 is a schematic view of the sealing element of FIG. 4 in a second stage;

FIG. 6 is a schematic view of the sealing member of FIG. 4 at a third stage;

FIG. 7 is a schematic view of the sealing element of FIG. 4 in a fourth stage;

FIG. 8 is a perspective view of the cup body and a cross-sectional view of the cup body;

FIG. 9 is a schematic structural view of a sealing member;

FIG. 10 is a schematic view of the base in one orientation;

fig. 11 is a schematic view of the structure of the base in another direction.

Detailed Description

The structures referred to in the present invention or these terms of art used are further described below, and if not otherwise indicated, they are understood and explained by general terms commonly used in the art.

Detection of

Detection refers to assaying or testing for the presence of a substance or material, such as, but not limited to, a chemical, organic compound, inorganic compound, metabolic product, drug or drug metabolite, organic tissue or a metabolite of organic tissue, nucleic acid, protein, or polymer. In addition, detection indicates the amount of the test substance or material. Further, the assay means immunodetection, chemical detection, enzyme detection, and the like.

Sample(s)

The test device or collected sample of the present invention comprises a biological fluid (e.g., a medical fluid or a clinical sample). Liquid or liquid samples, or fluid samples, may be derived from solid or semi-solid samples, including fecal, biological tissue and food samples. The solid or semi-solid sample may be converted to a liquid sample by any suitable method, such as mixing, triturating, macerating, incubating, dissolving, or enzymatically digesting a solid sample in a suitable solution (e.g., water, phosphate solution, or other buffered solution). "biological samples" include samples derived from animals, plants and food, including, for example, urine, saliva, blood and components thereof, spinal fluid, vaginal secretions, sperm, feces, sweat, secretions, tissues, organs, tumors, cultures, cell cultures and media of tissues and organs derived from humans or animals. Preferably, the biological sample is urine and preferably, the biological sample is saliva. Food samples include food processing materials, end products, meat, cheese, wine, milk and drinking water. Plant samples include those derived from any plant, plant tissue, plant cell culture and medium. An "environmental sample" is derived from the environment (e.g., a liquid sample from a lake or other body of water, a sewage sample, a soil sample, groundwater, seawater, and a waste liquid sample). Environmental samples may also include sewage or other wastewater.

Utilize the utility model discloses suitable detecting element or test element can detect any analyte. Preferably utilizes the utility model discloses detect the drugs micromolecule in saliva, urine. Of course, any of the above forms of samples, whether initially solid or liquid, may be collected using the collection device of the present invention, provided that the liquid or liquid sample is absorbed by the absorbent member. Absorbent members herein are generally made of a water-absorbent material that is initially dry and capable of absorbing a liquid or fluid sample by capillary or other properties of the absorbent member material. The absorbent material may be any material capable of absorbing liquid, such as sponge, filter paper, polyester fiber, gel, nonwoven fabric, cotton, polyester film, yarn, and the like. Of course the absorbent member need not be made of absorbent material and may be made of non-absorbent material, but rather the absorbent member has holes, threads, cavities therein, and samples, typically solid or semi-solid samples, may be collected on such structures and filled between the threads, the holes, or the pores.

Downstream and upstream

Downstream or upstream is divided with respect to the direction of liquid flow, typically liquid flows from upstream to downstream regions. The downstream region receives liquid from the upstream region, and liquid may also flow along the upstream region to the downstream region. It is also generally divided in the direction of liquid flow, for example, on materials that use capillary forces to urge liquid flow, the liquid may flow by gravity in the opposite direction to gravity, and in this case, the upstream and downstream are also divided in the direction of liquid flow.

Gas or liquid communication

By gas or liquid communication is meant that liquid or gas can flow from one place to another, possibly guided by some physical structure during the flow. By physical structures is generally meant that the liquid flows passively or actively to another place through the surface of the physical structures or the space inside the physical structures, and passively is generally a flow caused by external force, such as a flow under capillary action. The flow here can also be a liquid or a gas, because of its own effect (gravity or pressure), or a passive flow. Communication herein does not necessarily mean that a liquid or gas is required to be present, but merely that in some cases a connection or condition between two objects, if any, may flow from one object to the other. This refers to a state in which two objects are connected, and conversely, if there is no liquid communication or gas communication between the two objects, if there is liquid in or on one object, the liquid cannot flow into or on the other object, and such a state is a state of non-communication, non-liquid or gas communication.

Test element

The term "test element" as used herein refers to an element that can detect whether a sample or specimen contains an analyte of interest, and the detection can be based on any technical principles, such as immunology, chemistry, electricity, optics, molecular, nucleic acid, physics, etc. The test element may be a lateral flow test strip which detects a plurality of analytes. Of course, other suitable test elements may be used with the present invention.

Various test elements may be combined and used in the present invention. One form is a test strip. Test strips for the analysis of analytes, such as drugs or metabolites indicative of a physical condition, in a sample may be in various forms, such as immunoassay or chemical assay forms. The test strip may be used in a non-competitive or competitive assay format. The test strip generally comprises a bibulous material having a sample application area, a reagent area, and a test area. The sample is added to the sample application zone and flows by capillary action to the reagent zone. In the reagent zone, the sample binds to the reagent if the analyte is present. The sample then continues to flow to the detection zone. Other reagents, such as molecules that specifically bind to the analyte, are immobilized at the detection zone. These reagents react with the analyte (if present) in the sample and bind the analyte to the zone, or to one of the reagents of the reagent zone. The label for indicating the detection signal is present in the reagent zone or in a separate label zone.

A typical non-competitive assay format is one in which a signal is generated if the sample contains the analyte and no signal is generated if the analyte is not present. In a competition method, a signal is generated if the analyte is not present in the sample and no signal is generated if the analyte is present.

The test element can be a test paper, and can be made of water-absorbing or non-water-absorbing materials. The test strip may include a variety of materials for liquid sample delivery. One of the test strips may be coated with another material, such as a nitrocellulose membrane coated with filter paper. One region of the test strip may be selected from one or more materials and another region may be selected from a different one or more materials. The test strip may be adhered to some support or hard surface for improved strength when the test strip is held in place.

The analyte is detected by a signal producing system, such as one or more enzymes that specifically react with the analyte, and one or more compositions of the signal producing system are immobilized on the analyte detection zone of the test strip by a method such as that described above for the immobilization of a specific binding substance on the test strip. The signal-producing substance can be on the sample addition zone, reagent zone, or detection zone, or the entire test strip, and the substance can be impregnated on one or more materials of the test strip. A solution containing the signal is applied to the surface of the strip or one or more materials of the strip are immersed in the solution containing the signal. The strip to which the solution containing the signal substance was added was dried.

The various regions of the test strip may be arranged as follows: the device comprises a sample adding area, a reagent area, a detection area, a control area, a sample adulteration area and a liquid sample absorption area. The control zone is located behind the detection zone. All zones may be arranged on a strip of test paper using only one material. It is also possible to use different materials for the different zones. The zones may be in direct contact with the liquid sample, or different zones may be arranged according to the direction of flow of the liquid sample, with the ends of each zone being contiguous with and overlapping the ends of the other zone. The material used can be a material with good water absorption such as filter paper, glass fiber or nitrocellulose membrane. The test strip may take other forms.

A commonly used reagent strip is a nitrocellulose membrane reagent strip, i.e., a detection area comprises a nitrocellulose membrane, and a specific binding molecule is fixed on the nitrocellulose membrane to display the detection result; and may be a cellulose acetate film, a nylon film, or the like. Such as the reagent strips or devices containing the reagent strips described in some of the following patents: US 4857453; US 5073484; US 5119831; US 5185127; US 5275785; US 5416000; US 5504013; US 5602040; US 5622871; US 5654162; US 5656503; US 5686315; US 5766961; US 5770460; US 5916815; US 5976895; US 6248598; US 6140136; US 6187269; US 6187598; US 6228660; US 6235241; US 6306642; US 6352862; US 6372515; US 6379620; and US 6403383. The test strip disclosed in the above patent documents and similar devices with test strips can be applied to the test element or the test device of the present invention for detecting an analyte, such as an analyte in a sample.

The test strips used in the present invention may be so-called Lateral flow test strips (Lateral flow test strips), and the specific structure and detection principle of these test strips are well known in the art. A typical test strip comprises a sample collection area or application area, a labeling area comprising a label pad, a detection area comprising a bibulous pad, and a bibulous area comprising the necessary chemicals to detect the presence of the analyte, such as immunological or enzymatic reagents. A commonly used detection reagent strip is a nitrocellulose membrane reagent strip, that is, a detection area comprises a nitrocellulose membrane, and a specific binding molecule is fixed on the nitrocellulose membrane to display a detection result; it may be a cellulose acetate film, a nylon film, etc., and it may also include a detection result control region downstream of the detection region, and usually, the control region and the detection region are in the form of a transverse line, which is a detection line or a control line. Such test strips are conventional, but other types of test strips that utilize capillary action for testing are also contemplated. In addition, typically, the test strip has a dry chemical reagent component, such as an immobilized antibody or other reagent, which when exposed to a liquid, flows along the test strip by capillary action, and as it flows, the dry reagent component is dissolved in the liquid, and the next zone is processed to react the dry reagent in that zone, thereby performing the necessary test. The liquid flow is mainly by capillary action. The present invention can be applied to a detecting device, or can be disposed in a detecting chamber to contact with a liquid sample, or can be used to detect whether an analyte exists or the amount of the analyte exists in the liquid sample entering the detecting chamber.

In addition to the test strips described above or the lateral flow test strip itself being used to contact a liquid sample to test for the presence of an analyte. In some preferred forms, the test element may also be provided on a carrier having a plurality of recesses in which the test element is located. In some embodiments, the carrier includes a recessed area for receiving the test elements, and a plurality of recesses are provided in the recessed area, each of which can receive a test strip, and each of which can detect an analyte. In some embodiments, after the test elements are disposed in the recesses of the carrier, the carrier is covered with a transparent film, which seals the recess area of the carrier and facilitates viewing of the test results on the final test area. The transparent film may also be a transparent plastic sheet, transparent only in the test area.

Typically, the test strip includes a sample application region, a labeling region and a detection region, the sample application region being positioned adjacent to the bottom of the carrier and slightly exposing the recess, for example 2-3 mm, when the test strip is placed, with a portion of the sample application region reserved to absorb fluid sample flowing into the bottom of the collection chamber. Typically, the sample application zone is located upstream of the labeling zone, which is located upstream of the detection zone.

Such carriers are useful for carrying test strips in applications where these particular carriers may be used as part of the assay in the assay chamber of the invention, such as described in DE19780221T1, JP1999506213A, US6702988, US7244392, US20040133128A, US20070065339A 1.

Analyte substance

Examples of analytes that can be used in the present invention include small molecule substances, including drugs of abuse (e.g., drugs of abuse). By "drug of abuse" (DOA) is meant the use of a drug (usually acting to paralyze nerves) at a non-medical destination. Abuse of these drugs can result in physical and mental damage, dependence, addiction and/or death. Examples of drug abuse include cocaine; amphetamine AMP (e.g., black americane, white amphetamine tablets, dextroamphetamine tablets, Beans); methamphetamine MET (crank, methamphetamine, crystal, speed); barbiturate BAR (e.g., Valium, Roche Pharmaceuticals, Nutley, New Jersey); sedatives (i.e., sleep-aid drugs); lysergic acid diethylamide (LSD); inhibitors (downs, goofballs, barbs, blue devils, yellow jacks, hypnones); tricyclic antidepressants (TCAs, i.e., imipramine, amitriptyline and doxepin); dimethyldioxymethylaniline MDMA; phencyclidine (PCP); tetrahydrocannabinol (THC, pot, dope, hash, weed, etc.); opiates (i.e., morphine, or opiates, cocaine, COC; heroin, dihydrocodeinone); anxiolytic and sedative hypnotic, anxiolytic is a kind of mainly used for relieving anxiety, stress, fear, stabilize mood, have hypnotic sedative effects at the same time, including benzodiazepine BZO (benzodiazepines), atypical BZ, fuse dinitrogen NB23C, benzodiazepine, BZ receptor ligand, ring-opening BZ, diphenylmethane derivatives, piperazine carboxylate, piperidine carboxylate, quinazolone, thiazine and thiazole derivatives, other heterocycles, imidazole type sedative/analgesic (such as dihydrocodeinone OXY, methadone MTD), propylene glycol derivative-carbamate, aliphatic compound, anthracene derivatives, etc.. The detection device of the utility model can also be used for detecting the detection which belongs to the medical purpose and is easy to take excessive medicine, such as tricyclic antidepressants (imipramine or analogues) and acetaminophen, etc. After being absorbed by human body, the medicines are metabolized into small molecular substances, and the small molecular substances exist in body fluids such as blood, urine, saliva, sweat and the like or exist in partial body fluids.

For example, analytes detected using the present invention include, but are not limited to, creatinine, bilirubin, nitrite, protein (non-specific), hormones (e.g., human chorionic gonadotropin, progesterone hormone, follicle stimulating hormone, etc.), blood, leukocytes, sugars, heavy metals or toxins, bacterial material (e.g., proteins or carbohydrate material directed against specific bacteria, such as, e.g., Escherichia coli 0157: H7, staphylococci, Salmonella, Clostridium, Campylobacter, L. monocytogenes, Vibrio, or Cactus), and substances associated with physiological characteristics in urine samples, such as pH and specific gravity. Any other clinical urine chemical analysis can all utilize the cooperation of side direction crossing current detection form the utility model discloses the device detects.

Flow of liquid

The flow of liquid usually refers to a flow from one place to another, and in general, the natural liquid flow mostly depends on gravity from high to low, and the flow here also depends on external force, i.e. the flow under the external gravity condition, and can be the natural gravity flow. In addition to gravity, the flow of liquid may also overcome gravity and move from low to high. For example, the liquid is pumped, or the liquid is compressed, or the liquid is pressurized and flows from the bottom to the top, or the pressure is concerned and flows by the gravity of the liquid itself.

Mixing cavity and detection cavity

The mixed cavity is filled with a detection liquid, the mixed cavity is a cavity for mixing the sample and the detection liquid, and the sample and the detection liquid are dissolved in the detection liquid after being mixed to obtain a mixed liquid. When no sample is added into the mixing cavity, the detection cavity is not communicated with the mixing cavity; and adding a sample into the mixing cavity, and after a period of time, dissolving the sample in the detection liquid, wherein the mixing cavity and the detection cavity can be communicated through external force. The position that general detection chamber set up is less than the hybrid chamber, or the position that the detection chamber set up is the same with the hybrid chamber height on the horizontal direction, become when the hybrid chamber becomes the connected state by non-connected state between the detection chamber, the mixed liquid of hybrid chamber inside can flow in under the effect of gravity and detect the intracavity, there is test element in the detection chamber, test element can detect whether there is the analyte matter in the mixed liquid, intercommunication and non-intercommunication between detection chamber and the hybrid chamber are controlled through sealing element, sealing element includes two operating position at least: the sealing element comprises a first working position and a second working position, wherein when the sealing element is in the first working position, the mixing cavity and the detection cavity are in a non-communication state; when the sealing element is in the second working position, the mixing chamber is in a state of communication with the detection chamber. Specifically, referring to fig. 3 to 9, the detector main body 30 includes a mixing chamber 10 and a detection chamber 20, a detection liquid is pre-filled in the mixing chamber 10, a test strip 21 is filled in the detection chamber 20, the bottoms of the mixing chamber 10 and the detection chamber 20 are located on the same horizontal plane, a first through hole 31 is formed in a position, close to the bottom, of the inner wall between the mixing chamber 10 and the detection chamber 20, a sealing element 40 is assembled in the first through hole 31, the sealing element 40 has elasticity, and the sealing element 40 is preferably a sealing plug made of silicone. The inner wall of the detection chamber 20 is provided with a second communication hole 39 corresponding to the first communication hole 31, and the sealing member 40 extends to the outside of the detector body 30 through the second communication hole 39. In some forms, and with reference to fig. 4 and 9, the sealing element 40 is provided with a groove 45, the width of the groove 45 being greater than the wall thickness between the mixing chamber 10 and the detection chamber 20. The groove 45 divides the sealing element 40 into two parts: a first sealing portion 46 and a second sealing portion 47, in fig. 4, the first sealing portion 46 seals the first communication hole 31, the second sealing portion 47 seals the second communication hole 39, the mixing chamber 10 and the detection chamber 20 are in a non-communication state, and the sealing element 40 is in the first working position and is also in the initial state of the sealing element 40. Referring to fig. 5, when the sealing element 40 is subjected to an external force, the sealing element 40 moves, the first sealing portion 46 is offset from the first communication hole 31, the first communication hole 31 is no longer sealed, the gap between the groove 45 and the first communication hole 31 can communicate the mixing chamber 10 and the detection chamber 20, the second sealing portion 47 still seals the second communication hole 39, the detection chamber 20 is still in a non-communication state with the outside, and the sealing element 40 is in the second working position. In some preferred embodiments, referring to fig. 4 and 9, the sealing element 40 is further provided with a first annular protrusion 43 and a second annular protrusion 44, and the first annular protrusion 43 and the second annular protrusion 44 are respectively located at the left and right sides of the groove 45. When the sealing element 40 is in an initial state (the sealing element 40 is not subjected to external force, and the mixing chamber 10 and the detection chamber 20 are in a non-communicated state), the first annular bulge 43 is tightly attached to the inner wall of the mixing chamber 10, the second annular bulge 44 is tightly attached to the outer wall of the detection chamber 20, the first annular bulge 43 and the second annular bulge 44 limit the sealing element 40 from the left side and the right side respectively, so that the sealing element 40 is not easy to move inwards or outwards, and the mixing chamber 10 and the detection chamber 20 are always in a non-communicated state without the external force. The change of the working position of the sealing member 40 is described in detail below.

The first stage is as follows: when the operator needs to perform the sample detection, the operator firstly adds the sample into the mixing chamber 10 to mix with the detection liquid, and when the sample is dissolved in the detection liquid, referring to fig. 4 and 5, the sealing element 40 is moved towards the inside of the detector main body 30 by pressing the portion of the sealing element 40 located at the outer side of the detector main body 30, in the process, since the second annular protrusion 44 is tightly attached to the outer wall of the detection chamber 20 in the initial state, the second annular protrusion 44 needs to be deformed and inserted into the second communication hole 39, and the sealing element 40 can move, in the process, the operator obviously feels that a large force is needed to press the sealing element 40 at the beginning.

And a second stage: referring to fig. 5, when the second annular projection 44 of the sealing element 40 has been inserted into the second communication hole 39, the sealing element 40 is displaced by a force that is mainly: the friction between the second sealing portion 47 and the second communication hole 39 and the friction between the deformed second annular projection 44 and the second communication hole 39, however, the force to be overcome in this process is already much smaller than the force required to press the deformed second annular projection 44 into the second communication hole 39 in the first stage. And the force in the second stage is almost constant, the force in the first stage is abrupt, and the operator can easily perceive it by hand feeling. In the second stage, the first sealing portion 46 is separated from the first communication hole 31 along with the movement of the sealing element 40, and at this time, the mixed liquid in the mixing chamber 10 slowly flows into the detection chamber 20 through the gap formed between the groove 45 and the first communication hole 31 under the action of gravity, the test strip 21 in the detection chamber 20 detects the analyte of the mixed liquid, and the test strip generally comprises a sample application area, a marking area and a detection area, wherein the sample application area is located upstream of the marking area, the marking area is located upstream of the detection area, when the test strip is placed, the sample application area is placed at the bottom of the detection chamber 20, the mixed liquid enters the detection chamber 20 and then contacts with the sample application area (the lower end of the test strip 21), and the lower end of the mixed liquid contacting the test strip 21 starts to flow from bottom to top by virtue of capillary force.

The process of the operator pressing the sealing element 40 from the first stage to the second stage is actually the transition of the sealing element 40 from the first working position to the second working position, and generally, the sealing element 40 only needs to have two working positions, namely the first working position and the second working position, so that the basis of sample detection is provided.

And a third stage: referring to fig. 6, as the sealing member 40 continues to move, the second annular projection 44 comes out of the second communication hole 39 into the detection chamber 20, and the second annular projection 44 returns to its original state, during which the operator can sense a slight shaking of the sealing member 40 by hand feeling, which is caused by the rapid return elastic deformation of the second annular projection 44 at the moment when the second annular projection 44 comes out of the second communication hole 39. At the same time, during the period after the second annular projection 44 comes out of the second communication hole 39, the movement of the sealing element 40 becomes easier, because the force to be overcome to push the sealing element 40 to move is only: the friction between the second sealing portion 47 and the second communication hole 39 is much smaller in the third stage than in the second stage, in which the mixing chamber 10 and the detection chamber 20 are still in communication through the gap formed between the groove 45 and the first communication hole 31, and generally, up to the third stage, the operator does not press the sealing member 40 any more.

The sealing element 40 is still in the second working position during the process of pressing the sealing element 40 by the hand of the operator from the second stage to the third stage, the third stage being present in order to remind the operator that the mixing chamber 10 is in communication with the detection chamber 20, and the pressing of the sealing element 40 can be stopped.

A fourth stage: referring to fig. 7, the fourth stage is formed by the operator pressing the sealing member 40 too much, when the second sealing portion 47 of the sealing member 40 has completely entered the second communication hole 39, it is inconvenient to continue pressing the sealing member 40, and the left side of the second sealing portion 47 abuts against the first communication hole 31, the sealing member 40 is in the third working position, and the mixing chamber 10 and the detecting chamber 20 become non-communicated again. If the sealing element 40 continues to be pressed into the device after the sealing element 40 reaches the third working position, at this time, since the left side of the second sealing portion 47 abuts against the first communication hole 31, the force required for continuing to press is suddenly increased relative to the force at the third stage, and the operator is reminded to stop pressing. In the fourth stage, the second sealing portion 47 of the sealing member 40 still seals the second communication hole 39 to prevent the mixed liquid in the detection chamber 20 from leaking to the outside of the apparatus.

The setting of fourth stage is mainly in order to remind operating personnel not to excessively press sealing element 40, lets sealing element 40 seal first through-hole 31 once more simultaneously, lets mixing chamber 10 and detection chamber 20 become the non-connected state, because when mixing chamber 10 and detection chamber 20 were in the connected state all the time, the mixed liquid that flows into in the detection chamber 20 probably had too much circumstances, and the mixed liquid is crossed the sample on the test strip and is applyed the region, influences the testing result. In some preferred embodiments, by controlling the volume of the test solution added to the mixing chamber 10, the mixture does not overflow the sample application area on the test strip even though the mixing chamber 10 and the detection chamber 20 are always in communication.

In summary, the force for pressing the sealing member 40 is always reduced in the first stage to the third stage, and the force for pressing the sealing member 40 is suddenly increased in the third stage to the fourth stage, so that there are various methods for distinguishing whether the sealing member 40 is pressed completely: 1. the force experienced during the compression process suddenly increases, meaning that the fourth phase has been entered and the compression is immediately stopped. It is observed that the second sealing portion 47 of the sealing member 40 has completely entered the second communication hole 39, and the pressing is stopped immediately. 3. The pressing may be stopped by sensing the shaking of the sealing member 40 during the pressing. 4. During the pressing, the continuity of the pressing force decreases, and the sealing member 40 has mostly entered the second communication hole 39, the pressing may be stopped. Meanwhile, in the process from the first stage to the fourth stage, the position of the sealing element 40 after pressing the sealing element 40 is not reversible, that is, the process of the sealing element 40 transforming from the first working position to the second working position or from the second working position to the third working position is not reversible, and in general, the sealing element 40 cannot transform from the third working position to the second working position or from the second working position to the first working position, which is shown in fig. 1 because the end of the sealing element 40 exposed out of the device is a smooth surface, and the sealing element 40 is hard to be stressed when the operator pulls out the sealing element 40, unlike the pressing of the sealing element 40. Furthermore, if the sealing element 40 is already in the second operating position, the second sealing element 40 is now pulled out to be brought into the first operating position again, which is of no practical significance. Because the mixed liquid already flows into the detection chamber when the sealing element 40 is in the second working position, at which point the sealing element 40 is forcibly pulled out from the second working position to the first working position, mixed liquid is still present in the detection chamber, even if the device returns to the first working position, the device cannot be used for secondary detection, if the outward pulling operation is to change the mixing chamber 10 and the detection chamber 20 from the communication state to the non-communication state (to avoid too much mixed liquid flowing into the detection chamber 20), the sealing element 40 is selected to continuously press the sealing element 40 to change the sealing element 40 to the third working position when the sealing element 40 is in the second working position, both can achieve the same purpose, and the technical means adopted by the latter is relatively easy, in general, the transition of the sealing element 40 from the first operating position into the second operating position or from the second operating position into the third operating position is therefore irreversible.

In some preferred modes, the detector main body 30 is formed by assembling a cup body 32 and a base 33 together and then ultrasonically welding, wherein the cup body 32 comprises a first opening 34 with an upward opening and a second opening 35 with a downward opening, the first opening 34 is communicated with the second opening 35, and a missing area 36 is further arranged on the side surface of the cup body 32; base 33 includes collet 37 and side cap 38, when cup body 32 and base 33 accomplish the welding, second opening 35 and collet 37 have constituted hybrid chamber 10, missing area 36 and side cap 38 have constituted detection chamber 20, be equipped with two first protruding strips 22 that are used for fixed test strip 21 in the detection chamber 20, be equipped with fixed closed angle 23 on the relative one side of first protruding strip 22, test strip 21 is fixed in between two first protruding strips 22 through fixed closed angle 23, because the test strip is rectangular form generally, still be equipped with two protruding strips 24 of second in the detection chamber 20, first protruding strip 22 and the protruding strip 24 of second are used for the both ends of fixed test strip 21 respectively. In some forms, the first and second raised

strips

22, 24 may be provided on the wall of the absent area 36 of the cup body 32, or on the inside of the side cover 38 of the base 33.

In some preferred modes, referring to fig. 11, the side cover 38 is provided with a sliding slot 41, and the sliding slot 41 allows the cup body 32 to slide down along the sliding slot 41 during the assembly process of the cup body 32 and the base 33, so that the cup body 32 is in close contact with the base 33.

In some preferred modes, the cup body 32 adopts opaque material to once process the shaping through the mould, base 33 adopts transparent material to once process the shaping through the mould, like this when cup body 32 and base 33 assemble together back through ultrasonic welding as an organic whole, the lateral wall of hybrid chamber 10 is opaque, can avoid operating personnel to directly see some samples that have pollution nature with the naked eye, for example the shit, the lateral wall of detection chamber 20 is transparent, make things convenient for operating personnel direct observation test strip 21's mark region, transparent base 33 makes things convenient for operating personnel to observe the state of sealing element 40 simultaneously, whether the observation mixed liquid gets into in the detection chamber 20.

In some preferred embodiments, referring to fig. 10, the outer wall of the side cover 38 is provided with a raised area 50 near the second communication hole 39, the raised area 50 surrounds the second communication hole 39, and referring to fig. 1 and 3, when the sealing element 40 is installed in the second communication hole 39, the raised area 50 can prevent the sealing element 40 from moving toward the inside of the detector main body 30 due to a violent collision of the detection device during transportation, and if the mixing chamber 10 is communicated with the detection chamber 20 when no sample is added, and the detection liquid directly flows into the detection chamber 20, the detection device is discarded.

In some preferred embodiments, referring to fig. 11, a thickened wall 51 is provided inside the side cover 38 at the position of the second communication hole 39, and the thickened wall 51 can increase the depth of the second communication hole 39, so that the second sealing portion 47 always contacts with the second communication hole 39 during the process of pressing the sealing element 40 by the operator, thereby preventing the mixed liquid in the detection chamber 20 from leaking.

Sample collector

The sample collector is used for collecting samples, and referring to fig. 2 and 3 specifically, the sample collector 70 includes a connecting end 71, a rod 72, and a sampling end 73, wherein the connecting end 71 is detachably connected to the rod 72, and the rod 72 and the sampling end 73 are integrally formed. In some embodiments, the connecting end 71 has a connecting hole at the lower end thereof for matching with the rod 72, and the rod 72 can be inserted into the connecting hole to connect with the connecting end 71. In some embodiments, the sampling end 73 is divided into two types, which are respectively used for sampling a solid sample and a liquid sample, and referring to fig. 2, the sampling end 73 is in a spoon shape, and is provided with a sieve hole therein, which is used for sampling the solid sample, and the sieve hole can filter out liquid contained in the solid sample; the sampling end 73 is spoon-shaped, and no sieve holes are arranged in the sampling end, so that the sampling end can be used for sampling liquid samples.

Sample cavity and cover

The sample chamber is a chamber body (only capable of storing solid samples) capable of adding quantitative samples into the mixing chamber and storing a part of samples, and the position of the sample chamber is generally located above the mixing chamber because the mixing chamber is internally provided with detection liquid, and if the sample chamber is located below the mixing chamber, the situation that the detection liquid in the mixing chamber leaks into the sample chamber may exist, and the pollution of the reserved samples can be caused. Referring to fig. 2-3 and 8 specifically, the sample chamber 60 is located above the mixing chamber 10, specifically, the sample chamber 60 is located in the cup body 32 near the first opening 34, the mixing chamber 10 is located in the cup body 32 near the second opening 35, the sample chamber 60 is located directly above the mixing chamber 10, a partition board 61 is disposed between the sample chamber 60 and the mixing chamber 10, a sample adding hole 62 is disposed in the partition board 61, the sample adding hole 62 communicates the sample chamber 60 with the mixing chamber 10, and the size of the sample adding hole 62 matches with the sample collector. In some embodiments, when the solid sample is collected by the sample collector 70, the solid sample is collected by the screened sampling end 73 and then the sample is added into the mixing chamber 10 through the sample adding hole 62, the sample adding hole 62 can only pass a certain amount of the solid sample, and the excessive solid sample is blocked by the partition plate 61 and remains in the sample chamber 60. In other embodiments, when the liquid sample is collected by the sample collector 70, the liquid sample is collected by the sampling end 73 without a mesh and then poured into the sample adding hole 62, the sample passes through the sample adding hole 62 and enters the mixing chamber 10, and the amount of the liquid sample is controlled by the sampling end 73, for example, 10ml of the liquid sample needs to be added into the mixing chamber 10, and 5ml of the liquid sample can be sampled by one sampling end 73, so that only two times of sampling is needed.

In some preferred manners, the position of the sample application hole 62 on the partition plate 61 is recessed downward, the sample application hole 62 is the lowest position on the partition plate 61, the downward recess is designed to guide the sample application device 70 during the downward insertion of the sample application device 70, the sample application device 70 can be easily inserted without intentionally aligning the sample application device 70 with the sample application hole 62, and in addition, when the sample application device 70 is used for applying a liquid sample, only the liquid sample needs to be added into the sample cavity 60, and the liquid sample can flow into the sample application hole 62 along the partition plate 61, thereby facilitating the sampling of the liquid sample.

The cover body is a device for sealing the sample cavity, and the cover body and the sample cavity can be covered or separated. In the sampling process, the cover body and the sample cavity are in a separated state, so that a sample collector can conveniently add a sample into the sample cavity; in the process of detecting the analysis substance, the cover body and the sample cavity are in a covering state, so that some samples with odor can be prevented from emitting odor. Referring to fig. 2-3, the shape of the cover 80 matches the first opening 34 of the cup body 32, the cover 80 includes an outer wall 81 and an inner wall 82, the outer wall 81 and the inner wall 82 form a certain included angle, and the distance between the outer wall 81 and the inner wall 82 at the upper side of the cover 80 is smaller than the distance between the outer wall 81 and the inner wall 82 at the lower side of the cover 80, by pressing the cover 80 downward, the wall at the position of the first opening 34 of the cup body 32 can be clamped into the gap between the outer wall 81 and the inner wall 82 of the cover 80, and as the cover 80 covers the cup body 32 downward, since the distance between the outer wall 81 and the inner wall 82 on the cover 80 is always decreased, the cover 80 and the cup body 32 are more and more tightly covered. In some preferred modes, referring to fig. 8, a covering protrusion 83 is disposed on the cup body 32 at the position of the first opening 34, the covering protrusion 83 is in an inverted triangle shape, and the covering protrusion 83 can be embedded between the outer wall 81 and the inner wall 82 of the cover body 80 during the covering process of the cup body 32 and the cover body 80, so as to increase the deformation between the outer wall 81 and the inner wall 82, thereby increasing the clamping force between the outer wall 81 and the inner wall 82 and making the covering more tight.

In some preferred embodiments, the connection end 71 is integrally formed with the cover 80, and the connection end 71 is located at the center of the cover 80, and correspondingly, the position of the sample adding hole 62 in the cup body 32 corresponds to the connection end 71, so that the connection end 71 can always pass through the sample adding hole 62 without distinguishing the orientation of the cover 80 during the process of covering the cover 80 and the sample chamber 60.

When the sample detection device of the utility model is applied to the fecal occult blood detection project, the community residents can easily complete self-detection at home; meanwhile, the sample detection device of the utility model can avoid the direct vision and contact of community residents with excrement in the detection process, and can isolate the odor of the excrement, so that the detection process is clean and sanitary, and residents are willing to carry out self-detection; in the detection process, the sampling amount is not required to be controlled, the obtained detection result is very visual, and the self comparison of residents is facilitated; the sample can be stayed to the sample to device inside, makes things convenient for the resident to carry the excrement sample to the hospital and carries out the secondary inspection.

The above description is only the specific embodiments of the present invention, but the protection scope of the present invention is not limited thereto, and any changes or substitutions that are not thought of through creative work should be covered within the protection scope of the present invention, and therefore, the protection scope of the present invention should be subject to the protection scope defined by the claims.

The utility model shown and described herein may be implemented in the absence of any element, limitation, or limitations specifically disclosed herein. The terms and expressions which have been employed are used as terms of description and not of limitation, and there is no intention in the use of such terms and expressions of excluding any equivalents of the features shown and described or portions thereof, and it is recognized that various modifications are possible within the scope of the invention. It should therefore be understood that although the present invention has been specifically disclosed by various embodiments and optional features, modification and variation of the concepts herein described may be resorted to by those skilled in the art, and that such modifications and variations are considered to be within the scope of this invention as defined by the appended claims.

The contents of the articles, patents, patent applications, and all other documents and electronically available information described or cited herein are hereby incorporated by reference in their entirety to the same extent as if each individual publication was specifically and individually indicated to be incorporated by reference. Applicants reserve the right to incorporate into this application any and all materials and information from any such articles, patents, patent applications, or other documents.

Claims

1. A sample detector is characterized by comprising a mixing cavity, a detection cavity and a sealing element, wherein detection liquid is filled in the mixing cavity, a sample can be added into the mixing cavity, and after the sample is added, the detection liquid and the sample are mixed to obtain mixed liquid;

the sealing element comprises two operating positions: the sealing element comprises a first working position and a second working position, wherein when the sealing element is in the first working position, the mixing cavity and the detection cavity are in a non-communication state; when the sealing element is in the second working position, the mixing chamber is in a state of communication with the detection chamber.

2. A sample detector as claimed in claim 1 wherein the sealing member is resilient.

3. The sample detector as claimed in claim 1, wherein the sealing member is provided with a groove for communicating the mixing chamber with the detection chamber when the sealing member is in the second operating position.

4. The sample detector of claim 1, wherein the sealing member further comprises a third operative position, and wherein the mixing chamber is not in communication with the detection chamber when the sealing member is in the third operative position.

5. A sample detector as claimed in claim 4 wherein the transition of the sealing member from the first to the second operating position or from the second to the third operating position is irreversible.

6. The sample detector as claimed in claim 1, wherein the sealing member comprises a first sealing portion, and a first communication hole is formed between the mixing chamber and the detection chamber;

7. A sample detector as claimed in claim 4 or 6 wherein the sealing member further comprises a second sealing portion which seals the first aperture when the sealing member is in the third operating position.

8. The sample detector as claimed in claim 7, wherein the detecting chamber is provided with a second sealing hole communicated with the outside, and when the sealing member is at the first operating position, the second operating position or the third operating position, the second sealing portion always seals the second sealing hole.

9. The sample detector of claim 1, wherein the sealing member defines a first annular protrusion and a second annular protrusion, the first annular protrusion engaging the inner wall of the mixing chamber and the second annular protrusion engaging the outer wall of the detection chamber when the sealing member is in the first operating position.

10. A sample detector as claimed in claim 8 or 9 wherein the first annular projection is located at the first sealing region and the second annular projection is located at the second sealing region.