WO2021036368A1 - Epidermis fungus sampling and staining method - Google Patents
Epidermis fungus sampling and staining method Download PDFInfo
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- WO2021036368A1 WO2021036368A1 PCT/CN2020/092135 CN2020092135W WO2021036368A1 WO 2021036368 A1 WO2021036368 A1 WO 2021036368A1 CN 2020092135 W CN2020092135 W CN 2020092135W WO 2021036368 A1 WO2021036368 A1 WO 2021036368A1
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- sampling
- transparent
- viscous material
- material layer
- comb
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- 238000005070 sampling Methods 0.000 title claims abstract description 80
- 241000233866 Fungi Species 0.000 title claims abstract description 46
- 238000007447 staining method Methods 0.000 title claims abstract description 9
- 210000002615 epidermis Anatomy 0.000 title abstract 4
- 238000001514 detection method Methods 0.000 claims abstract description 49
- 239000011345 viscous material Substances 0.000 claims abstract description 37
- 238000012360 testing method Methods 0.000 claims abstract description 13
- 238000012546 transfer Methods 0.000 claims abstract description 12
- 238000010186 staining Methods 0.000 claims abstract description 9
- XLYOFNOQVPJJNP-UHFFFAOYSA-N water Chemical compound O XLYOFNOQVPJJNP-UHFFFAOYSA-N 0.000 claims abstract description 8
- 239000008367 deionised water Substances 0.000 claims abstract description 7
- 229910021641 deionized water Inorganic materials 0.000 claims abstract description 7
- 239000000243 solution Substances 0.000 claims description 42
- NIXOWILDQLNWCW-UHFFFAOYSA-N acrylic acid group Chemical group C(C=C)(=O)O NIXOWILDQLNWCW-UHFFFAOYSA-N 0.000 claims description 28
- 238000004043 dyeing Methods 0.000 claims description 28
- 238000000034 method Methods 0.000 claims description 25
- KWYUFKZDYYNOTN-UHFFFAOYSA-M Potassium hydroxide Chemical compound [OH-].[K+] KWYUFKZDYYNOTN-UHFFFAOYSA-M 0.000 claims description 24
- PEDCQBHIVMGVHV-UHFFFAOYSA-N Glycerine Chemical compound OCC(O)CO PEDCQBHIVMGVHV-UHFFFAOYSA-N 0.000 claims description 16
- JVTAAEKCZFNVCJ-UHFFFAOYSA-N lactic acid Chemical compound CC(O)C(O)=O JVTAAEKCZFNVCJ-UHFFFAOYSA-N 0.000 claims description 16
- 230000001681 protective effect Effects 0.000 claims description 15
- 238000007689 inspection Methods 0.000 claims description 12
- ZXJXZNDDNMQXFV-UHFFFAOYSA-M crystal violet Chemical compound [Cl-].C1=CC(N(C)C)=CC=C1[C+](C=1C=CC(=CC=1)N(C)C)C1=CC=C(N(C)C)C=C1 ZXJXZNDDNMQXFV-UHFFFAOYSA-M 0.000 claims description 8
- YQGOJNYOYNNSMM-UHFFFAOYSA-N eosin Chemical compound [Na+].OC(=O)C1=CC=CC=C1C1=C2C=C(Br)C(=O)C(Br)=C2OC2=C(Br)C(O)=C(Br)C=C21 YQGOJNYOYNNSMM-UHFFFAOYSA-N 0.000 claims description 8
- 229960001235 gentian violet Drugs 0.000 claims description 8
- 235000011187 glycerol Nutrition 0.000 claims description 8
- 239000004310 lactic acid Substances 0.000 claims description 8
- 235000014655 lactic acid Nutrition 0.000 claims description 8
- 239000011259 mixed solution Substances 0.000 claims description 8
- 238000000386 microscopy Methods 0.000 abstract description 2
- 208000001840 Dandruff Diseases 0.000 abstract 3
- 239000000975 dye Substances 0.000 abstract 1
- 238000004659 sterilization and disinfection Methods 0.000 abstract 1
- 238000005406 washing Methods 0.000 abstract 1
- 239000011521 glass Substances 0.000 description 13
- 239000000463 material Substances 0.000 description 8
- 230000000694 effects Effects 0.000 description 5
- 241000555676 Malassezia Species 0.000 description 4
- 239000000203 mixture Substances 0.000 description 3
- 239000002245 particle Substances 0.000 description 3
- 210000004761 scalp Anatomy 0.000 description 3
- 239000012780 transparent material Substances 0.000 description 3
- 239000000853 adhesive Substances 0.000 description 2
- 230000001070 adhesive effect Effects 0.000 description 2
- 210000001520 comb Anatomy 0.000 description 2
- 238000011109 contamination Methods 0.000 description 2
- SMZOUWXMTYCWNB-UHFFFAOYSA-N 2-(2-methoxy-5-methylphenyl)ethanamine Chemical compound COC1=CC=C(C)C=C1CCN SMZOUWXMTYCWNB-UHFFFAOYSA-N 0.000 description 1
- 208000025309 Hair disease Diseases 0.000 description 1
- 240000007594 Oryza sativa Species 0.000 description 1
- 235000007164 Oryza sativa Nutrition 0.000 description 1
- 230000009286 beneficial effect Effects 0.000 description 1
- 230000034303 cell budding Effects 0.000 description 1
- 235000013339 cereals Nutrition 0.000 description 1
- 238000004140 cleaning Methods 0.000 description 1
- 230000007547 defect Effects 0.000 description 1
- 230000001419 dependent effect Effects 0.000 description 1
- 238000003745 diagnosis Methods 0.000 description 1
- 238000009792 diffusion process Methods 0.000 description 1
- 238000010828 elution Methods 0.000 description 1
- 230000002538 fungal effect Effects 0.000 description 1
- 210000003128 head Anatomy 0.000 description 1
- 239000006210 lotion Substances 0.000 description 1
- 238000012986 modification Methods 0.000 description 1
- 230000004048 modification Effects 0.000 description 1
- 238000011022 operating instruction Methods 0.000 description 1
- 238000004806 packaging method and process Methods 0.000 description 1
- 230000002265 prevention Effects 0.000 description 1
- 238000012545 processing Methods 0.000 description 1
- 230000033458 reproduction Effects 0.000 description 1
- 235000009566 rice Nutrition 0.000 description 1
- 208000017520 skin disease Diseases 0.000 description 1
- 238000009827 uniform distribution Methods 0.000 description 1
- 239000002699 waste material Substances 0.000 description 1
Images
Classifications
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- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N1/00—Sampling; Preparing specimens for investigation
- G01N1/28—Preparing specimens for investigation including physical details of (bio-)chemical methods covered elsewhere, e.g. G01N33/50, C12Q
- G01N1/30—Staining; Impregnating ; Fixation; Dehydration; Multistep processes for preparing samples of tissue, cell or nucleic acid material and the like for analysis
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N1/00—Sampling; Preparing specimens for investigation
- G01N1/28—Preparing specimens for investigation including physical details of (bio-)chemical methods covered elsewhere, e.g. G01N33/50, C12Q
- G01N1/30—Staining; Impregnating ; Fixation; Dehydration; Multistep processes for preparing samples of tissue, cell or nucleic acid material and the like for analysis
- G01N2001/302—Stain compositions
Definitions
- the invention belongs to the technical field of fungal detection and processing, and in particular relates to a method for sampling and dyeing epidermal fungi.
- epidermal fungi plays an important guiding role in the diagnosis and prevention of skin and hair diseases.
- direct sampling and staining microscopy is one of the fastest judgment methods, and it can also provide key guidance information for further culture identification.
- the traditional method of epidermal sampling is to scrape the dander from the test site with a scalpel or the end of a glass slide, collect it in an appropriate package, and then transfer it to the laboratory, where it is stained on the glass slide for microscopic examination.
- This method of sampling and staining has the following defects: (1) Sampling of the head skin is not suitable for use with razor blades or glass slides in areas with hair; (2) The scraped sample needs to be transferred with packaging, and multiple transfers may easily lose the sample. (3) The dander sample is difficult to fix after being transferred to the glass slide, and it is washed away by the dye and lotion during the dyeing process, causing the sample to be lost. The dyeing operation is difficult; (4) The sample is heavy.
- Swarf and fungus will be dyed at the same time. Even if a specific dye is used, it is difficult to distinguish dander and fungus in color, which makes it difficult to identify the fungus attached or hidden in the dander. In addition, the entire sampling and dyeing is very dependent on the experience and level of the operator.
- the present invention provides a method for sampling and dyeing epidermal fungi.
- a method for sampling and dyeing epidermal fungi including the following steps:
- Step S01. Provide a transparent detection card, the transparent detection card has a detection area, the detection area is attached with a layer of transparent viscous material, and the surface of the transparent viscous material layer is covered with a protective film;
- Step S02. Use a sterilized sampling comb to comb several times along the direction of the hair of the subject to be tested, so that the dander sticks to the sampling comb;
- Step S03. Remove the protective film on the transparent detection card, and repeatedly stick the tip of the sampling comb with dander on the surface of the transparent viscous material layer, so that a sufficient amount of dander sticks to the transparent On the viscous material layer;
- Step S04. Drop A dye solution on the surface of the transparent viscous material layer, and then add the same amount of B dye solution as the A dye solution on the surface of the transparent viscous material layer, and use deionized water after standing still. rinse;
- Step S05 Transfer the transparent inspection card to a microscope for microscopic examination to obtain information on dander and fungus.
- the epidermal fungus sampling and dyeing method provided by the present invention directly transfers the sample obtained by the sampling comb to the transparent test card, which is convenient for sampling, easy to transfer and not easy to be contaminated, and easy to fix and not easy to dye and clean.
- the elution and dyeing time is short, which improves the success rate and efficiency of sampling and dyeing.
- Figure 1 is a schematic top view of a transparent detection card of the present invention
- Figure 2 is a schematic cross-sectional view taken along line A-A of Figure 1;
- Figure 3 shows the effect of sampling and dyeing epidermal fungi using conventional sampling and dyeing methods
- Fig. 4 shows the dyeing effect of sampling and dyeing epidermal fungi in Example 1 of the present invention
- Fig. 5 shows the dyeing effect of sampling and dyeing epidermal fungi in Example 2 of the present invention
- Fig. 6 shows the dyeing effect of sampling and dyeing epidermal fungi in Example 3 of the present invention
- 100-transparent detection card 1-transparent area, 2-label area; 11-detection area; 111-transparent adhesive material layer, 112-protective film.
- the invention provides a method for sampling and dyeing epidermal fungi.
- the method for sampling and dyeing epidermal fungi needs to involve a transparent detection card 100.
- the transparent detection card 100 includes a transparent area 1 and a label area 2.
- the transparent area 1 is fixed with a detection area 11, and the detection area 11 is pasted with a transparent viscous material layer 111, and a protective film 112 is pasted directly above the transparent viscous material layer 111 to prevent the transparent viscous material layer 111 from being contaminated before use, and the protective film 112 should be removed during use;
- the label area 2 can be used to paste information of the person to be tested, and the operator can hold the label area 2 for easy operation.
- the above-mentioned transparent inspection card 100 is divided into a transparent area 1 and a label area 2. It does not mean that only the transparent area 1 is transparent. It is mainly used to distinguish two different areas.
- the entire transparent inspection card 100 is made of transparent material.
- the label area 2 can be a non-transparent material.
- the above-mentioned epidermal fungus sampling and staining method includes the following steps:
- Step S01. Provide a transparent detection card 100 as shown in Figures 1 and 2;
- Step S02. Use a sterilized sampling comb to comb several times along the direction of the hair of the subject to be tested, so that the dander sticks to the sampling comb;
- Step S03. Remove the protective film 112 on the transparent detection card 100, and repeatedly stick the tip of the sampling comb with dander on the surface of the transparent viscous material layer, so that a sufficient amount of dander sticks to the surface of the transparent viscous material layer.
- Step S04. Drop A dye solution on the surface of the transparent viscous material layer, and then add the same amount of B dye solution as the A dye solution on the surface of the transparent viscous material layer, and use deionized water after standing still. rinse;
- Step S05 Transfer the transparent inspection card to a microscope for microscopic examination to obtain information on dander and fungus.
- the viscous material used for the viscous material layer 111 is preferably acrylic.
- Acrylic is a transparent material that will not be dyed by the dye solution. Observe the morphology of the sample clearly under the microscope.
- the area of the transparent detection area 11 is (70-350) mm 2 , and the transparent detection area 11 may be a square area, a circular area, or the like. More preferably, it is a circular area, and the area and the circular area are conducive to the adhesion of the epidermal sample, the uniform distribution and diffusion of the dye solution, and the use of the dye solution can be reduced.
- the thickness of the transparent viscous material layer 111 is (0.5 ⁇ 1.5) mm. After the thickness is not suitable, the adhesion of the epidermal sample will not be improved after the thickness exceeds 1.5 mm. Instead, acrylic acid will be wasted, which is too thin, such as thickness. If it is less than 0.5 mm, the sampling comb is likely to directly damage the transparent viscous material layer 111.
- the sampling comb is a plastic comb, that is, a common plastic comb. It is better to have special hand-held and non-hand-held parts for the sampling comb, so as not to interfere with the sampling by external factors such as hands during the sampling process or even contaminate the obtained skin .
- the sampling comb is placed in different positions along the direction of the subject’s hair for 3 to 5 times.
- combing try to keep only one side of the comb and the tip of the comb during combing. To touch the scalp, but avoid excessive force to cause damage to the scalp. If the comb sticks to the hair, use tweezers to remove the hair on the comb surface, and avoid touching the tips of the teeth when removing the hair with tweezers to avoid sample loss.
- sampling After sampling, if you do not directly perform on-site testing, you can store the sampling comb in a clean sealed bag and store it in a cool and dry environment.
- the storage time should be less than one week as much as possible, and the test should be performed within one week.
- step S03 when transferring the obtained skin sample to the transparent detection card 100, the protective film 112 on the surface of the detection area is first removed.
- the protective film 112 avoid touching the viscous material layer 111 to avoid contamination.
- the dye solution A is a mixed solution of eosin and potassium hydroxide, and the mass concentration of eosin in the mixed solution is 0.8% to 1.2%, and the mass concentration of potassium hydroxide is 8.5% to 12.5% .
- the mass concentration of eosin may be 1.0%, and the mass concentration of potassium hydroxide may be 10%.
- the B dye solution is a three-mixed solution of gentian violet, lactic acid and glycerin, and the mass concentration of gentian violet in the three-mixed solution is 0.8% to 1.5%, the mass concentration of lactic acid is 18% to 25%, and glycerin The mass concentration of 15% to 25%.
- the mass concentration of gentian violet in the B dye solution can be 1.0%
- the mass concentration of lactic acid can be 20%
- the mass concentration of glycerin can be 20%.
- the A dye solution is dripped onto the surface of the viscous material layer 111, and then the B dye solution in the same amount as the A dye solution is dripped onto the surface of the viscous material layer 111, and the dyeing can be completed after standing for 10 to 15 seconds. Ionized water cleaning.
- the dripping amount of the A dye solution is (80-120) ⁇ L; the dripping amount of the B dye solution is (80-120) ⁇ L.
- the dripping amount is too small to be able to dye completely, and the dripping amount is too much, resulting in waste.
- step S05 microscope inspection, please refer to the microscope manual for specific operation methods.
- the stained transparent inspection card 100 is stuck on the microscope stage with the inspection area 11 facing up, move the inspection area 11 to just below the lens, observe with a 10x objective lens, and locate the area where the dander is attached. Turn to 40x and fine-tune the focus until a clear picture is presented. Note: When adjusting the stage up and down, especially when using a 40x objective lens, be careful to avoid the detection area from contacting the objective lens.
- a method for sampling and dyeing epidermal fungi including the following steps:
- the transparent detection card made of glass, the transparent detection card has a detection area, the detection area is attached with a layer of acrylic, the acrylic layer is circular, the thickness is 1mm, and the area is 153.86mm 2 , the The surface of the acrylic layer is covered with a protective film;
- a dye solution formed of eosin with a mass concentration of 1.0% and potassium hydroxide with a mass concentration of 10% on the surface of the acrylic layer drop 100 ⁇ L, and then mix with the A dye solution.
- a quantity of B dye solution in B dye solution, the mass concentration of gentian violet is 1.0%, the mass concentration of lactic acid is 20%, and the mass concentration of glycerin is 20%) are dropped on the surface of the acrylic layer, and after standing for 15 seconds Rinse with deionized water;
- the test result is shown in Figure 4.
- the dander Under the 10x objective lens, the dander can be seen, most of which are transparent, and a small part of it is dyed blue-purple.
- small particles can be seen around the dander, zoomed in to 40 times, you can see that the particles dyed in blue-purple are rice grains, and some particles have small protrusions at one end, which is typical For Malassezia, part A represents free Malassezia, part B represents sterile dander, and part C represents a large number of fungi attached to the dander.
- a method for sampling and dyeing epidermal fungi including the following steps:
- the transparent detection card made of glass, the transparent detection card has a detection area, the detection area is attached with a layer of acrylic, the acrylic layer is circular, the thickness is 0.5mm, the area is 346.18mm 2 , so The surface of the acrylic layer is covered with a protective film;
- a dye solution formed of eosin with a mass concentration of 1.2% and potassium hydroxide with a mass concentration of 10% on the surface of the acrylic layer drop 100 ⁇ L, and then mix with the A dye solution.
- a quantity of B dye solution in B dye solution, the mass concentration of gentian violet is 0.8%, the mass concentration of lactic acid is 18%, and the mass concentration of glycerin is 15%) is dropped on the surface of the acrylic layer, and after standing for 15s Rinse with deionized water;
- a sampling and staining method for epidermal fungi is performed by mailing sample combs.
- the transparent detection card made of glass, the transparent detection card has a detection area, the detection area is attached with a layer of acrylic, the acrylic layer is round, the thickness is 1.5mm, the area is 78.5mm 2 , so The surface of the acrylic layer is covered with a protective film;
- a dye solution formed of eosin with a mass concentration of 0.8% and potassium hydroxide with a mass concentration of 12.5% on the surface of the acrylic layer drop 100 ⁇ L, and then mix with the A dye solution.
- a quantity of B dye solution in the B dye solution, the mass concentration of gentian violet is 0.8%, the mass concentration of lactic acid is 25%, and the mass concentration of glycerin is 25%) are dropped on the surface of the acrylic layer, and after standing for 15 seconds Rinse with deionized water;
- test results are shown in Figure 6. It can be seen from Fig. 6 that at 40 times, a large number of spherical and rice-shaped fungi stained blue can be seen around transparent or light blue dander, which are preliminarily determined to be two fungi belonging to the genus Malassezia by morphology. At the same time, it was proved that the sampling comb was stored at room temperature for one week after sampling, and no impact on the test results was found.
Abstract
An epidermis fungus sampling and staining method. The epidermis fungus sampling and staining method comprises: providing a transparent detection card (100) having a detection area (11), a transparent viscous material layer (111) being attached to the detection area (11), and a surface of the transparent viscous material layer (111) being covered with a protection film (112); combing in the hair direction of a subject under test for multiple times by using a sampling comb subjected to disinfection treatment, so that dandruff is sticked to the sampling comb; uncovering the protection film (112) on the transparent detection card (100), and repeatedly attaching tooth tips where the dandruff is sticked of the sampling comb to the surface of the transparent viscous material layer (111) to enable sufficient dandruff to be sticked to the transparent viscous material layer (111); sequentially dropwise adding equal amounts of dyes A and B to the surface of the transparent viscous material layer (111), standing, and washing with deionized water; and transferring the transparent detection card (100) under a microscope for microscopy. The epidermis fungus sampling and staining method has the characteristics that sampling is convenient, samples are easy to transfer and fix and not easy to pollute, the staining time is short, and the like, and the success rate and efficiency of sampling and staining are improved.
Description
本发明属于真菌检测处理技术领域,具体涉及一种表皮真菌取样染色方法。The invention belongs to the technical field of fungal detection and processing, and in particular relates to a method for sampling and dyeing epidermal fungi.
表皮的真菌检测对于皮肤、毛发的疾病诊断和预防有着重要的指导作用。其中,直接取样染色镜检是最为快速的判断方法之一,还可以为进一步的培养鉴定提供关键的指导信息。The detection of epidermal fungi plays an important guiding role in the diagnosis and prevention of skin and hair diseases. Among them, direct sampling and staining microscopy is one of the fastest judgment methods, and it can also provide key guidance information for further culture identification.
传统的表皮取样方法是用手术刀或者载玻片末端刮取测试部位的皮屑,收集于适当的包装内,然后转移至实验室,并在载玻片上染色镜检。这种取样和染色方法存在以下缺陷:(1)头部皮肤的取样在有头发的部位不适合用刀片或者载玻片;(2)刮取的样品需要用包装转移,多次转移容易损失样品和混入污染物;(3)皮屑样品转移至载玻片后难以固定,在染色过程中被染液和洗液冲走导致样品丢失,是的染色操作难度大;(4)样品重的皮屑和真菌会被同时染色,即使使用特定的染液,也难以在颜色上显著区分皮屑和真菌,导致附着或者隐藏于皮屑之中的真菌难以识别。此外,整个取样染色非常依赖操作人员的经验、水平。The traditional method of epidermal sampling is to scrape the dander from the test site with a scalpel or the end of a glass slide, collect it in an appropriate package, and then transfer it to the laboratory, where it is stained on the glass slide for microscopic examination. This method of sampling and staining has the following defects: (1) Sampling of the head skin is not suitable for use with razor blades or glass slides in areas with hair; (2) The scraped sample needs to be transferred with packaging, and multiple transfers may easily lose the sample. (3) The dander sample is difficult to fix after being transferred to the glass slide, and it is washed away by the dye and lotion during the dyeing process, causing the sample to be lost. The dyeing operation is difficult; (4) The sample is heavy. Swarf and fungus will be dyed at the same time. Even if a specific dye is used, it is difficult to distinguish dander and fungus in color, which makes it difficult to identify the fungus attached or hidden in the dander. In addition, the entire sampling and dyeing is very dependent on the experience and level of the operator.
发明概述Summary of the invention
问题的解决方案The solution to the problem
针对目前表皮真菌取样染色存在取样难度大、样品容易被污染、染色操作难且样品易丢失、不易区分皮屑和真菌等问题,本发明提供一种表皮真菌取样染色方法。Aiming at the problems of high sampling difficulty in sampling and dyeing of epidermal fungi, easy contamination of samples, difficult dyeing operations, easy loss of samples, and difficulty in distinguishing dander and fungi, the present invention provides a method for sampling and dyeing epidermal fungi.
为实现上述发明目的,本发明的技术方案如下:In order to achieve the above-mentioned purpose of the invention, the technical scheme of the present invention is as follows:
一种表皮真菌取样染色方法,包括以下步骤:A method for sampling and dyeing epidermal fungi, including the following steps:
步骤S01.提供透明检测卡,所述透明检测卡上具有检测区域,所述检测区域附着有一层透明粘性材料层,且所述透明粘性材料层表面覆盖有一层保护膜;Step S01. Provide a transparent detection card, the transparent detection card has a detection area, the detection area is attached with a layer of transparent viscous material, and the surface of the transparent viscous material layer is covered with a protective film;
步骤S02.采用经过消毒处理的取样梳顺着待测试者的头发方向梳若干次,使得皮屑粘在所述取样梳上;Step S02. Use a sterilized sampling comb to comb several times along the direction of the hair of the subject to be tested, so that the dander sticks to the sampling comb;
步骤S03.揭去所述透明检测卡上的保护膜,将所述取样梳粘有皮屑的齿尖反复粘靠在所述透明粘性材料层表面,使得足够量的皮屑粘在所述透明粘性材料层上;Step S03. Remove the protective film on the transparent detection card, and repeatedly stick the tip of the sampling comb with dander on the surface of the transparent viscous material layer, so that a sufficient amount of dander sticks to the transparent On the viscous material layer;
步骤S04.将A染液滴加于所述透明粘性材料层表面,随后将与所述A染液等量的B染液滴加在所述透明粘性材料层表面,静置后采用去离子水冲洗;Step S04. Drop A dye solution on the surface of the transparent viscous material layer, and then add the same amount of B dye solution as the A dye solution on the surface of the transparent viscous material layer, and use deionized water after standing still. rinse;
步骤S05.将所述透明检测卡转移至显微镜下进行镜检,获取皮屑和真菌信息。Step S05. Transfer the transparent inspection card to a microscope for microscopic examination to obtain information on dander and fungus.
本发明的技术效果为:The technical effects of the present invention are:
相对于现有技术,本发明提供的表皮真菌取样染色方法,由于直接将取样梳获得的样品转移至透明检测卡上,取样方便、样品易于转移不易被污染并且样品易于被固定并且染色和清洗不易洗脱,同时染色时间短,提高了取样染色的成功率和效率。Compared with the prior art, the epidermal fungus sampling and dyeing method provided by the present invention directly transfers the sample obtained by the sampling comb to the transparent test card, which is convenient for sampling, easy to transfer and not easy to be contaminated, and easy to fix and not easy to dye and clean. The elution and dyeing time is short, which improves the success rate and efficiency of sampling and dyeing.
发明的有益效果The beneficial effects of the invention
对附图的简要说明Brief description of the drawings
为了更清楚地说明本发明实施例中的技术方案,下面将对实施例中所需要使用的附图作简单地介绍,显而易见地,下面描述中的附图仅仅是本发明的一些实施例,对于本领域普通技术人员来讲,在不付出创造性劳动的前提下,还可以根据这些附图获得其他的附图。In order to explain the technical solutions in the embodiments of the present invention more clearly, the following will briefly introduce the drawings that need to be used in the embodiments. Obviously, the drawings in the following description are only some embodiments of the present invention. A person of ordinary skill in the art can obtain other drawings based on these drawings without creative work.
图1为本发明透明检测卡俯视示意图;Figure 1 is a schematic top view of a transparent detection card of the present invention;
图2为图1沿A-A线的剖视示意图;Figure 2 is a schematic cross-sectional view taken along line A-A of Figure 1;
图3为采用常规取样染色方法对表皮真菌进行取样染色的效果;Figure 3 shows the effect of sampling and dyeing epidermal fungi using conventional sampling and dyeing methods;
图4为本发明实施例1对表皮真菌进行取样染色的染色效果;Fig. 4 shows the dyeing effect of sampling and dyeing epidermal fungi in Example 1 of the present invention;
图5为本发明实施例2对表皮真菌进行取样染色的染色效果;Fig. 5 shows the dyeing effect of sampling and dyeing epidermal fungi in Example 2 of the present invention;
图6为本发明实施例3对表皮真菌进行取样染色的染色效果;Fig. 6 shows the dyeing effect of sampling and dyeing epidermal fungi in Example 3 of the present invention;
其中,100-透明检测卡,1-透明区域,2-标签区域;11-检测区域;111-透明粘性材料层,112-保护膜。Among them, 100-transparent detection card, 1-transparent area, 2-label area; 11-detection area; 111-transparent adhesive material layer, 112-protective film.
发明实施例Invention embodiment
为了使本发明的目的、技术方案及优点更加清楚明白,以下结合附图及实施例,对本发明进行进一步详细说明。应当理解,此处所描述的具体实施例仅用以解释本发明,并不用于限定本发明。In order to make the objectives, technical solutions, and advantages of the present invention clearer, the following further describes the present invention in detail with reference to the accompanying drawings and embodiments. It should be understood that the specific embodiments described herein are only used to explain the present invention, but not used to limit the present invention.
本发明提供一种表皮真菌取样染色方法。The invention provides a method for sampling and dyeing epidermal fungi.
详见图1、2,该表皮真菌取样染色方法需要涉及一种透明检测卡100,该透明检测卡100包括透明区域1和标签区域2,其中透明区域1上固定有检测区域11,该检测区域11上粘贴有透明粘性材料层111,并且在透明粘性材料层111正上方贴附有一层保护膜112,避免透明粘性材料层111在使用前被污染,在使用时,将保护膜112揭除;标签区域2可以用于粘贴待测试者的信息,并且操作人员可以手持标签区域2以便于操作。上述透明检测卡100分成透明区域1和标签区域2,并不是代表只有透明区域1是透明的,其主要是用于区分两个不同的区域,整个透明检测卡100都是透明的材质做成,当然标签区域2可以是非透明材质。See Figures 1 and 2 for details. The method for sampling and dyeing epidermal fungi needs to involve a transparent detection card 100. The transparent detection card 100 includes a transparent area 1 and a label area 2. The transparent area 1 is fixed with a detection area 11, and the detection area 11 is pasted with a transparent viscous material layer 111, and a protective film 112 is pasted directly above the transparent viscous material layer 111 to prevent the transparent viscous material layer 111 from being contaminated before use, and the protective film 112 should be removed during use; The label area 2 can be used to paste information of the person to be tested, and the operator can hold the label area 2 for easy operation. The above-mentioned transparent inspection card 100 is divided into a transparent area 1 and a label area 2. It does not mean that only the transparent area 1 is transparent. It is mainly used to distinguish two different areas. The entire transparent inspection card 100 is made of transparent material. Of course, the label area 2 can be a non-transparent material.
上述表皮真菌取样染色方法包括以下步骤:The above-mentioned epidermal fungus sampling and staining method includes the following steps:
步骤S01.提供如图1、2所述的透明检测卡100;Step S01. Provide a transparent detection card 100 as shown in Figures 1 and 2;
步骤S02.采用经过消毒处理的取样梳顺着待测试者的头发方向梳若干次,使得皮屑粘在所述取样梳上;Step S02. Use a sterilized sampling comb to comb several times along the direction of the hair of the subject to be tested, so that the dander sticks to the sampling comb;
步骤S03.揭去所述透明检测卡100上的保护膜112,将所述取样梳粘有皮屑的齿尖反复粘靠在所述透明粘性材料层表面,使得足够量的皮屑粘在所述透明粘性材料层上;Step S03. Remove the protective film 112 on the transparent detection card 100, and repeatedly stick the tip of the sampling comb with dander on the surface of the transparent viscous material layer, so that a sufficient amount of dander sticks to the surface of the transparent viscous material layer. The transparent adhesive material layer;
步骤S04.将A染液滴加于所述透明粘性材料层表面,随后将与所述A染液等量的B染液滴加在所述透明粘性材料层表面,静置后采用去离子水冲洗;Step S04. Drop A dye solution on the surface of the transparent viscous material layer, and then add the same amount of B dye solution as the A dye solution on the surface of the transparent viscous material layer, and use deionized water after standing still. rinse;
步骤S05.将所述透明检测卡转移至显微镜下进行镜检,获取皮屑和真菌信息。Step S05. Transfer the transparent inspection card to a microscope for microscopic examination to obtain information on dander and fungus.
下面对上述表皮真菌取样染色方法做进一步的解释说明。The following is a further explanation of the above-mentioned epidermal fungus sampling and staining method.
步骤S01中,粘性材料层111使用的黏性材料优选为丙烯酸,丙烯酸为透明材质,不会被染液染色,有弹性、粘性好,便于粘附表皮样品,并且表面光滑平整性好,方便在显微镜下清晰的观察样品的形态。进一步优选地,透明检测区域1 1的面积为(70~350)mm
2,该透明检测区域11可以是方形区域、圆形区域等。更为优选地为圆形区域,该面积和圆形区域有利于粘取表皮样品,有利于染液的均匀分布和扩散,还能减少染液的使用量。
In step S01, the viscous material used for the viscous material layer 111 is preferably acrylic. Acrylic is a transparent material that will not be dyed by the dye solution. Observe the morphology of the sample clearly under the microscope. Further preferably, the area of the transparent detection area 11 is (70-350) mm 2 , and the transparent detection area 11 may be a square area, a circular area, or the like. More preferably, it is a circular area, and the area and the circular area are conducive to the adhesion of the epidermal sample, the uniform distribution and diffusion of the dye solution, and the use of the dye solution can be reduced.
优选地,所述透明粘性材料层111的厚度为(0.5~1.5)mm,厚度不宜过后,超过1.5mm后对于表皮样品的粘附没有任何提高的作用,反而会浪费丙烯酸,太薄,如厚度小于0.5mm,取样梳容易直接破坏透明粘性材料层111。Preferably, the thickness of the transparent viscous material layer 111 is (0.5~1.5) mm. After the thickness is not suitable, the adhesion of the epidermal sample will not be improved after the thickness exceeds 1.5 mm. Instead, acrylic acid will be wasted, which is too thin, such as thickness. If it is less than 0.5 mm, the sampling comb is likely to directly damage the transparent viscous material layer 111.
步骤S02中,取样梳为塑料梳,即常见的塑料梳篦,最好取样梳有专门的手持部位和非手持部位,以免在取样过程中手等外界因素对取样造成干扰甚至污染取到的表皮样品。在取样过程中,取样梳顺着待测试者的头发方向在不同位置上3~5次,即可,梳发时,尽量保持始终只使用梳子的一侧,梳发过程中取样梳的齿尖要触及头皮,但避免用力过度导致头皮破损,如果梳子粘有头发,应当使用镊子取下梳子表面的头发,并且镊子取头发时应当避免触碰齿尖以免样品损失。In step S02, the sampling comb is a plastic comb, that is, a common plastic comb. It is better to have special hand-held and non-hand-held parts for the sampling comb, so as not to interfere with the sampling by external factors such as hands during the sampling process or even contaminate the obtained skin . In the sampling process, the sampling comb is placed in different positions along the direction of the subject’s hair for 3 to 5 times. When combing, try to keep only one side of the comb and the tip of the comb during combing. To touch the scalp, but avoid excessive force to cause damage to the scalp. If the comb sticks to the hair, use tweezers to remove the hair on the comb surface, and avoid touching the tips of the teeth when removing the hair with tweezers to avoid sample loss.
取样结束,如果不直接进行现场检测,可以将取样梳保存在干净的密封袋中,在阴凉干燥的环境下保存,保存时间尽量少于一周,在一周之内检测。After sampling, if you do not directly perform on-site testing, you can store the sampling comb in a clean sealed bag and store it in a cool and dry environment. The storage time should be less than one week as much as possible, and the test should be performed within one week.
步骤S03中,将取到的表皮样品转移至透明检测卡100上时,先揭除检测区域表面的保护膜112,揭除保护膜112时,应当避免触碰粘性材料层111,以免造成污染。将取样梳粘有皮屑的齿尖轻轻触碰粘性材料层111表面,取样梳来回触碰若干次,即可使得皮屑样品转移至粘性材料层111表面。如果皮屑样品量不够,还可以将取样梳其他部位平贴于粘性材料层111表面,或者进行二次取样。In step S03, when transferring the obtained skin sample to the transparent detection card 100, the protective film 112 on the surface of the detection area is first removed. When removing the protective film 112, avoid touching the viscous material layer 111 to avoid contamination. Lightly touch the tooth tip of the sampling comb with the dander on the surface of the viscous material layer 111, and touch the sampling comb back and forth several times to transfer the dander sample to the surface of the viscous material layer 111. If the amount of dander sample is insufficient, other parts of the sampling comb can be flatly attached to the surface of the viscous material layer 111, or secondary sampling can be performed.
步骤S04中,所述A染液为伊红和氢氧化钾的混合溶液,其所述混合溶液中伊红的质量浓度为0.8%~1.2%,氢氧化钾的质量浓度为8.5%~12.5%。具体地,A染液中,伊红的质量浓度可以是1.0%,氢氧化钾的质量浓度可以是10%。In step S04, the dye solution A is a mixed solution of eosin and potassium hydroxide, and the mass concentration of eosin in the mixed solution is 0.8% to 1.2%, and the mass concentration of potassium hydroxide is 8.5% to 12.5% . Specifically, in dye solution A, the mass concentration of eosin may be 1.0%, and the mass concentration of potassium hydroxide may be 10%.
所述B染液为龙胆紫、乳酸及甘油的三混溶液,且所述三混溶液中龙胆紫的质量浓度为0.8%~1.5%、乳酸的质量浓度为18%~25%、甘油的质量浓度为15%~25%。具体地,B染液中龙胆紫的质量浓度可以是1.0%、乳酸的质量浓度可以是20%、甘油的质量浓度可以是20%。The B dye solution is a three-mixed solution of gentian violet, lactic acid and glycerin, and the mass concentration of gentian violet in the three-mixed solution is 0.8% to 1.5%, the mass concentration of lactic acid is 18% to 25%, and glycerin The mass concentration of 15% to 25%. Specifically, the mass concentration of gentian violet in the B dye solution can be 1.0%, the mass concentration of lactic acid can be 20%, and the mass concentration of glycerin can be 20%.
具体是将A染液滴加至粘性材料层111表面,随后将与A染液等量的B染液滴加 至粘性材料层111表面,静置10s~15s即可完成染色,并且可以采用去离子水清洗。Specifically, the A dye solution is dripped onto the surface of the viscous material layer 111, and then the B dye solution in the same amount as the A dye solution is dripped onto the surface of the viscous material layer 111, and the dyeing can be completed after standing for 10 to 15 seconds. Ionized water cleaning.
优选地,所述A染液的滴加量为(80~120)μL;所述B染液的滴加量为(80~120)μL。滴加量太少,不能够完全染色,滴加量过多,造成浪费。Preferably, the dripping amount of the A dye solution is (80-120) μL; the dripping amount of the B dye solution is (80-120) μL. The dripping amount is too small to be able to dye completely, and the dripping amount is too much, resulting in waste.
步骤S05中,显微镜镜检,具体操作方法请参照显微镜使用手册。In step S05, microscope inspection, please refer to the microscope manual for specific operation methods.
如将染色后的透明检测卡100,检测区域11朝上卡在显微镜载物台上,将检测区域11移动至镜头正下方,先用10倍物镜观察,定位至有皮屑黏附的区域,然后转至40倍,微调焦距直至呈现一个清晰的画面,注意:调节载物台上下时,尤其使用40倍物镜时注意要避免检测区域接触到物镜。For example, if the stained transparent inspection card 100 is stuck on the microscope stage with the inspection area 11 facing up, move the inspection area 11 to just below the lens, observe with a 10x objective lens, and locate the area where the dander is attached. Turn to 40x and fine-tune the focus until a clear picture is presented. Note: When adjusting the stage up and down, especially when using a 40x objective lens, be careful to avoid the detection area from contacting the objective lens.
为更有效的说明本发明的技术方案,下面通过多个具体实施例说明。In order to more effectively illustrate the technical solution of the present invention, a number of specific embodiments are used to illustrate the following.
实施例1Example 1
一种表皮真菌取样染色方法,包括以下步骤:A method for sampling and dyeing epidermal fungi, including the following steps:
(1).提供玻璃材质的透明检测卡,所述透明检测卡上具有检测区域,所述检测区域附着有一层丙烯酸层,丙烯酸层呈圆形,厚度为1mm,面积为153.86mm
2,所述丙烯酸层表面覆盖有一层保护膜;
(1) Provide a transparent detection card made of glass, the transparent detection card has a detection area, the detection area is attached with a layer of acrylic, the acrylic layer is circular, the thickness is 1mm, and the area is 153.86mm 2 , the The surface of the acrylic layer is covered with a protective film;
(2).采用经过消毒处理的取样梳顺着待测试者的头发方向梳3次,每次梳头发的不同部位,使得皮屑粘在所述取样梳上;(2) Use a sterilized sampling comb to comb three times along the direction of the subject's hair, each time combing different parts of the hair, so that the dander sticks to the sampling comb;
(3).揭去玻璃材质透明检测卡上的保护膜,将所述取样梳粘有皮屑的齿尖粘靠于所述丙烯酸层表面,并将所述取样梳其他粘有皮屑的其他部位粘靠在所述丙烯酸层表面,使得足够量的皮屑粘在所述丙烯酸层上;(3). Remove the protective film on the glass material transparent detection card, stick the tip of the sampling comb with dander on the surface of the acrylic layer, and attach the sampling comb with other dander The parts stick to the surface of the acrylic layer, so that a sufficient amount of dander sticks to the acrylic layer;
(4).将由质量浓度为1.0%的伊红和质量浓度为10%的氢氧化钾形成的A染液滴加于所述丙烯酸层表面,滴加100μL,随后将与所述A染液等量的B染液(B染液中,龙胆紫的质量浓度为1.0%、乳酸的质量浓度为20%、甘油的质量浓度为20%)滴加在所述丙烯酸层表面,静置15s后采用去离子水冲洗;(4). Drop A dye solution formed of eosin with a mass concentration of 1.0% and potassium hydroxide with a mass concentration of 10% on the surface of the acrylic layer, drop 100 μL, and then mix with the A dye solution. A quantity of B dye solution (in B dye solution, the mass concentration of gentian violet is 1.0%, the mass concentration of lactic acid is 20%, and the mass concentration of glycerin is 20%) are dropped on the surface of the acrylic layer, and after standing for 15 seconds Rinse with deionized water;
(5).将所述玻璃材质透明检测卡转移至显微镜下进行镜检,获取皮屑和真菌信息;(5). Transfer the glass material transparent inspection card to a microscope for microscopic examination to obtain information on dander and fungus;
检测结果如图4所示,在10倍物镜下能看到皮屑,大部分为透明,少部分被染成蓝紫色。在有马拉色菌的样品中,能看到皮屑周围有细小颗粒,放大至40倍 ,可看到被染色成蓝紫色的颗粒呈米粒状,部分颗粒一端会有小突起,则为典型的马拉色菌,A部分表示游离的马拉色菌,B部分表示无菌的皮屑,C部分表示皮屑上附着大量真菌。The test result is shown in Figure 4. Under the 10x objective lens, the dander can be seen, most of which are transparent, and a small part of it is dyed blue-purple. In the sample with Malassezia, small particles can be seen around the dander, zoomed in to 40 times, you can see that the particles dyed in blue-purple are rice grains, and some particles have small protrusions at one end, which is typical For Malassezia, part A represents free Malassezia, part B represents sterile dander, and part C represents a large number of fungi attached to the dander.
而采用如背景技术里提到的常规取样染色方法对表皮真菌进行取样染色,染色结果如图3所示。从图3可知,皮屑同样被染色,并且率先被染色,导致真菌难以被识别。The conventional sampling and staining method as mentioned in the background art is used to sample and stain the epidermal fungus, and the staining result is shown in Figure 3. It can be seen from Figure 3 that the dander was also stained and was stained first, making it difficult to identify the fungus.
实施例2Example 2
一种表皮真菌取样染色方法,包括以下步骤:A method for sampling and dyeing epidermal fungi, including the following steps:
(1).提供玻璃材质的透明检测卡,所述透明检测卡上具有检测区域,所述检测区域附着有一层丙烯酸层,丙烯酸层呈圆形,厚度为0.5mm,面积为346.18mm
2,所述丙烯酸层表面覆盖有一层保护膜;
(1) Provide a transparent detection card made of glass, the transparent detection card has a detection area, the detection area is attached with a layer of acrylic, the acrylic layer is circular, the thickness is 0.5mm, the area is 346.18mm 2 , so The surface of the acrylic layer is covered with a protective film;
(2).采用经过消毒处理的取样梳顺着待测试者的头发方向梳3次,每次梳头发的不同部位,使得皮屑粘在所述取样梳上;(2) Use a sterilized sampling comb to comb three times along the direction of the subject's hair, each time combing different parts of the hair, so that the dander sticks to the sampling comb;
(3).揭去玻璃材质透明检测卡上的保护膜,将所述取样梳粘有皮屑的齿尖粘靠在所述丙烯酸层表面,并将所述取样梳其他粘有皮屑的其他部位粘靠在所述丙烯酸层表面,使得足够量的皮屑粘在所述丙烯酸层上;(3). Remove the protective film on the glass material transparent detection card, stick the tip of the sampling comb with dander on the surface of the acrylic layer, and put the sampling comb with other dander on the surface The parts stick to the surface of the acrylic layer, so that a sufficient amount of dander sticks to the acrylic layer;
(4).将由质量浓度为1.2%的伊红和质量浓度为10%的氢氧化钾形成的A染液滴加于所述丙烯酸层表面,滴加100μL,随后将与所述A染液等量的B染液(B染液中,龙胆紫的质量浓度为0.8%、乳酸的质量浓度为18%、甘油的质量浓度为15%)滴加在所述丙烯酸层表面,静置15s后采用去离子水冲洗;(4). Drop A dye solution formed of eosin with a mass concentration of 1.2% and potassium hydroxide with a mass concentration of 10% on the surface of the acrylic layer, drop 100 μL, and then mix with the A dye solution. A quantity of B dye solution (in B dye solution, the mass concentration of gentian violet is 0.8%, the mass concentration of lactic acid is 18%, and the mass concentration of glycerin is 15%) is dropped on the surface of the acrylic layer, and after standing for 15s Rinse with deionized water;
(5).将所述玻璃材质透明检测卡转移至显微镜下进行镜检,获取皮屑和真菌信息。(5). Transfer the glass material transparent inspection card to a microscope for microscopic examination to obtain information on dander and fungus.
检测结果如图5所示。从图5可知,40倍物镜下能清晰看到皮屑呈现透明或浅蓝色,周围存在大量被染成蓝色的球形真菌,并能看到出芽生殖迹象,经形态学初步判定为马拉色菌。The test results are shown in Figure 5. It can be seen from Figure 5 that under a 40x objective lens, the dander can be clearly seen as transparent or light blue, and there are a large number of spherical fungi dyed in blue around it, and signs of budding and reproduction can be seen. The morphology is preliminarily judged as Mala. Chromobacteria.
实施例3Example 3
一种表皮真菌取样染色方法,该实施例通过邮寄样品梳方式检测。A sampling and staining method for epidermal fungi. In this embodiment, the detection is performed by mailing sample combs.
(1).样品的获取:受测人因为不在本地,不方便当场检测,通过寄了一把清洁 消毒的样品梳,受测人本人用样品梳按本发明的操作说明梳过头皮后将样品梳放入无菌密封袋,常温保存,于一周内通过邮寄方式寄至检测实验室进行检测。(1). Obtaining samples: Because the subject is not in the local area, it is inconvenient to test on the spot. By sending a clean and disinfected sample comb, the subject himself uses the sample comb to comb the scalp according to the operating instructions of the present invention and then combs the sample. Put the comb into a sterile sealed bag, store it at room temperature, and send it to the testing laboratory for testing within one week by mail.
(2).提供玻璃材质的透明检测卡,所述透明检测卡上具有检测区域,所述检测区域附着有一层丙烯酸层,丙烯酸层呈圆形,厚度为1.5mm,面积为78.5mm
2,所述丙烯酸层表面覆盖有一层保护膜;
(2) Provide a transparent detection card made of glass, the transparent detection card has a detection area, the detection area is attached with a layer of acrylic, the acrylic layer is round, the thickness is 1.5mm, the area is 78.5mm 2 , so The surface of the acrylic layer is covered with a protective film;
(3).揭去玻璃材质透明检测卡上的保护膜,将所述取样梳粘有皮屑的齿尖粘靠在所述丙烯酸层表面,并将所述取样梳其他粘有皮屑的其他部位粘靠在所述丙烯酸层表面,使得足够量的皮屑粘在所述丙烯酸层上;(3). Remove the protective film on the glass material transparent detection card, stick the tip of the sampling comb with dander on the surface of the acrylic layer, and put the sampling comb with other dander on the surface The parts stick to the surface of the acrylic layer, so that a sufficient amount of dander sticks to the acrylic layer;
(4).将由质量浓度为0.8%的伊红和质量浓度为12.5%的氢氧化钾形成的A染液滴加于所述丙烯酸层表面,滴加100μL,随后将与所述A染液等量的B染液(B染液中,龙胆紫的质量浓度为0.8%、乳酸的质量浓度为25%、甘油的质量浓度为25%)滴加在所述丙烯酸层表面,静置15s后采用去离子水冲洗;(4). Drop A dye solution formed of eosin with a mass concentration of 0.8% and potassium hydroxide with a mass concentration of 12.5% on the surface of the acrylic layer, drop 100 μL, and then mix with the A dye solution. A quantity of B dye solution (in the B dye solution, the mass concentration of gentian violet is 0.8%, the mass concentration of lactic acid is 25%, and the mass concentration of glycerin is 25%) are dropped on the surface of the acrylic layer, and after standing for 15 seconds Rinse with deionized water;
(5).将所述玻璃材质透明检测卡转移至显微镜下进行镜检,获取皮屑和真菌信息。(5). Transfer the glass material transparent inspection card to a microscope for microscopic examination to obtain information on dander and fungus.
检测结果如图6所示。从图6可知在40倍下可以看到透明或浅蓝色皮屑周围有大量被染成蓝色的球形和米粒型真菌,经形态学初步判定为马拉色菌属的两种真菌。同时证明取样后取样梳常温保存一周,未发现对检测结果造成影响。The test results are shown in Figure 6. It can be seen from Fig. 6 that at 40 times, a large number of spherical and rice-shaped fungi stained blue can be seen around transparent or light blue dander, which are preliminarily determined to be two fungi belonging to the genus Malassezia by morphology. At the same time, it was proved that the sampling comb was stored at room temperature for one week after sampling, and no impact on the test results was found.
以上所述仅为本发明的较佳实施例而已,并不用以限制本发明,凡在本发明的精神和原则之内所作的任何修改、等同替换和改进等,均应包括在本发明的保护范围之内。The above are only the preferred embodiments of the present invention and are not intended to limit the present invention. Any modification, equivalent replacement and improvement made within the spirit and principle of the present invention shall be included in the protection of the present invention. Within range.
Claims (9)
- 一种表皮真菌取样染色方法,其特征在于,包括以下步骤:A method for sampling and dyeing epidermal fungi, which is characterized in that it comprises the following steps:步骤S01.提供透明检测卡,所述透明检测卡上具有检测区域,所述检测区域附着有一层透明粘性材料层,且所述透明粘性材料层表面覆盖有一层保护膜;Step S01. Provide a transparent detection card, the transparent detection card has a detection area, the detection area is attached with a layer of transparent viscous material, and the surface of the transparent viscous material layer is covered with a protective film;步骤S02.采用经过消毒处理的取样梳顺着待测试者的头发方向梳若干次,使得皮屑粘在所述取样梳上;Step S02. Use a sterilized sampling comb to comb several times along the direction of the hair of the subject to be tested, so that the dander sticks to the sampling comb;步骤S03.揭去所述透明检测卡上的保护膜,将所述取样梳粘有皮屑的齿尖反复粘靠在所述透明粘性材料层表面,使得足够量的皮屑粘在所述透明粘性材料层上;Step S03. Remove the protective film on the transparent detection card, and repeatedly stick the tip of the sampling comb with dander on the surface of the transparent viscous material layer, so that a sufficient amount of dander sticks to the transparent On the viscous material layer;步骤S04.将A染液滴加于所述粘性材料层表面,随后将与所述A染液等量的B染液滴加在所述透明粘性材料层表面,静置后采用去离子水冲洗;Step S04. Drop A dye solution on the surface of the viscous material layer, and then add the same amount of B dye solution as the A dye solution on the surface of the transparent viscous material layer, and rinse with deionized water after standing. ;步骤S05.将所述透明检测卡转移至显微镜下进行镜检,获取皮屑和真菌信息。Step S05. Transfer the transparent inspection card to a microscope for microscopic examination to obtain information on dander and fungus.
- 如权利要求1所述的表皮真菌取样染色方法,其特征在于,所述A染液为伊红和氢氧化钾的混合溶液,其所述混合溶液中伊红的质量浓度为0.8%~1.2%,氢氧化钾的质量浓度为8.5%~12.5%;The epidermal fungus sampling and staining method according to claim 1, wherein the A dye solution is a mixed solution of eosin and potassium hydroxide, and the mass concentration of eosin in the mixed solution is 0.8% to 1.2% , The mass concentration of potassium hydroxide is 8.5% ~ 12.5%;所述B染液为龙胆紫、乳酸及甘油的三混溶液,且所述三混溶液中龙胆紫的质量浓度为0.8%~1.5%、乳酸的质量浓度为18%~25%、甘油的质量浓度为15%~25%。The B dye solution is a three-mixed solution of gentian violet, lactic acid and glycerin, and the mass concentration of gentian violet in the three-mixed solution is 0.8% to 1.5%, the mass concentration of lactic acid is 18% to 25%, and glycerin The mass concentration of 15% to 25%.
- 如权利要求1所述的表皮真菌取样染色方法,其特征在于,所述A染液的滴加量为(80~120)μL;所述B染液的滴加量为(80~120)μL。The method for sampling and staining epidermal fungi according to claim 1, wherein the dripping amount of the A dye solution is (80-120) μL; the dripping amount of the B dye solution is (80-120) μL .
- 如权利要求1所述的表皮真菌取样染色方法,其特征在于,所述检测区域的面积为(70~350)mm 2。 The method for sampling and staining epidermal fungi according to claim 1, wherein the area of the detection area is (70-350) mm 2 .
- 如权利要求1所述的表皮真菌取样染色方法,其特征在于,所述透明粘性材料层的厚度为(0.5~1.5)mm。The method for sampling and dyeing epidermal fungi according to claim 1, wherein the thickness of the transparent viscous material layer is (0.5-1.5) mm.
- 如权利要求1所述的表皮真菌取样染色方法,其特征在于,所述透 明粘性材料层的粘性材料为丙烯酸。The method for sampling and dyeing epidermal fungi according to claim 1, wherein the viscous material of the transparent viscous material layer is acrylic.
- 如权利要求1所述的表皮真菌取样染色方法,其特征在于,所述取样梳为清洁消毒过的塑料梳。The method for sampling and dyeing epidermal fungi according to claim 1, wherein the sampling comb is a clean and disinfected plastic comb.
- 如权利要求1所述的表皮真菌取样染色方法,其特征在于,所述静置时间为(10~15)s。The method for sampling and staining epidermal fungi according to claim 1, wherein the standing time is (10-15) s.
- 如权利要求1所述的表皮真菌取样染色方法,其特征在于,所述透明检测卡还包括标签区,所述标签区用于标记待测试者的信息。The method for sampling and staining epidermal fungi according to claim 1, wherein the transparent detection card further comprises a label area, and the label area is used to mark the information of the test subject.
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