CN109609439A - Single celled method is separated from non-normal tissue - Google Patents

Single celled method is separated from non-normal tissue Download PDF

Info

Publication number
CN109609439A
CN109609439A CN201811594140.0A CN201811594140A CN109609439A CN 109609439 A CN109609439 A CN 109609439A CN 201811594140 A CN201811594140 A CN 201811594140A CN 109609439 A CN109609439 A CN 109609439A
Authority
CN
China
Prior art keywords
tissue
sample
digestive juice
normal tissue
method described
Prior art date
Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
Granted
Application number
CN201811594140.0A
Other languages
Chinese (zh)
Other versions
CN109609439B (en
Inventor
吴文铭
彭俊雅
陈澔
黄丹
刘路路
洪夏飞
丛林
李冬晶
赵玉沛
Current Assignee (The listed assignees may be inaccurate. Google has not performed a legal analysis and makes no representation or warranty as to the accuracy of the list.)
Peking Union Medical College Hospital Chinese Academy of Medical Sciences
Original Assignee
Peking Union Medical College Hospital Chinese Academy of Medical Sciences
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Application filed by Peking Union Medical College Hospital Chinese Academy of Medical Sciences filed Critical Peking Union Medical College Hospital Chinese Academy of Medical Sciences
Priority to CN201811594140.0A priority Critical patent/CN109609439B/en
Publication of CN109609439A publication Critical patent/CN109609439A/en
Application granted granted Critical
Publication of CN109609439B publication Critical patent/CN109609439B/en
Active legal-status Critical Current
Anticipated expiration legal-status Critical

Links

Classifications

    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N5/00Undifferentiated human, animal or plant cells, e.g. cell lines; Tissues; Cultivation or maintenance thereof; Culture media therefor
    • C12N5/06Animal cells or tissues; Human cells or tissues
    • C12N5/0602Vertebrate cells
    • C12N5/0676Pancreatic cells
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N2509/00Methods for the dissociation of cells, e.g. specific use of enzymes

Abstract

The present invention relates to unicellular separation field, discloses and separate single celled method from non-normal tissue.It is digested the described method includes: non-normal tissue's sample is mixed with digestive juice, the digestive juice contains VIII Collagenase Type, neutral proteinase, trypsin inhibitor and deoxyribonuclease, wherein, the ratio between the VIII Collagenase Type, neutral proteinase, trypsin inhibitor and the enzyme activity unit of deoxyribonuclease is 100-312.5:1-5:5000-25000:1.The present invention can realize that single celled high yield and high motility rate are extracted in the case where total digestion time is shorter, especially pancreatic tissue, capture the unicellular yield of existing pancreatic tissue and the lower problem of motility rate.

Description

Single celled method is separated from non-normal tissue
Technical field
The present invention relates to unicellular separation fields, and in particular to single celled method is separated from non-normal tissue.
Background technique
Pancreas is the organ that endocrine and exocrine function are had both in human body.It is thin comprising islet cells, acinus in histology Multiple cellular components such as born of the same parents, vessel cell and interstitial cell.Pancreas generates in the pancreatic juice of secretion containing trypsase, pancreas fat A variety of digestive ferments such as enzyme, amylopsin.With the rise of single cell analysis technology in recent years, people couple and human tissue organ Research is mixed from heterogeneity, and the global tissue analysis interfered with each other is gradually deep into the individual cells for constituting histoorgan Research, importance are self-evident.And in pancreas research field, due to pancreas organ's generally softness in fragile, histology Complicated component and it is easy to happen autodigestion because of potent pancreatin, so that pancreatic single cell research often stops at first Step --- namely the single celled acquisition of pancreatic tissue for analysis.
Human body or the unicellular separation method of animal model tissue organ are drawn from initial capillary, again to airflow classification To micro-fluidic technologies, numerous single-cell techniques more or less all achieves more satisfied knot in different tissues Fruit, but it is then barely satisfactory in pancreatic tissue.By consulting literatures it is found that researcher is slender in separating mouse cancer of pancreas at present When born of the same parents, the enzymic digestion dissociating method based on II Collagenase Type is mostly used greatly, and still, pancreatic single cell researcher indicates in pancreas Greatly challenge is encountered when the unicellular separation of gland or unicellular yield is not high or Cell viability is lower, therefore, exploitation The preparation or method for the pancreatic single cell that can be efficiently separated have particularly important meaning.
Summary of the invention
The purpose of the invention is to overcome the problems, such as that unicellular yield and Cell viability of the existing technology are lower, mention Single celled method is separated from non-normal tissue for a kind of new.
To achieve the goals above, the present invention provides one kind separates single celled method, the party from non-normal tissue Method includes: to mix non-normal tissue's sample with digestive juice to digest, and the digestive juice contains VIII Collagenase Type, neutral egg White enzyme, trypsin inhibitor and deoxyribonuclease, wherein the VIII Collagenase Type, neutral proteinase, trypsase Ratio between inhibitor and the enzyme activity unit of deoxyribonuclease is 100-312.5:1-5:5000-25000:1.
Through the above technical solutions, the present invention can realize single celled high yield in the case where total digestion time is shorter It is extracted with high motility rate, is based particularly on the unicellular separation of pancreatic tissue, has captured the unicellular yield of existing pancreatic tissue and work The lower problem of rate specifies direction for the single celled separation of pancreatic tissue, may advantageously facilitate to the further of pancreatic tissue Research.
Detailed description of the invention
Fig. 1 is to separate single celled result figure from pancreatic tissue using the method for specific embodiment according to the present invention;
Fig. 2 to Fig. 5 is to separate single celled result figure from pancreatic tissue using different reference methods respectively.
Specific embodiment
The endpoint of disclosed range and any value are not limited to the accurate range or value herein, these ranges or Value should be understood as comprising the value close to these ranges or value.For numberical range, between the endpoint value of each range, respectively It can be combined with each other between the endpoint value of a range and individual point value, and individually between point value and obtain one or more New numberical range, these numberical ranges should be considered as specific open herein.
In the present invention, in the absence of explanation to the contrary, term " enzyme activity unit " reaction used is that enzyme contains Amount number, refer under given conditions, converted in 1 minute in 1 micromole substrate or substrate needed for the related group of 1 micromole Enzyme amount, referred to as an enzyme activity unit (IU, also known as U).
Wherein, the definition of the enzyme activity unit of VIII Collagenase Type is: under conditions of pH 7.5 and 37 DEG C, hydrolysis in 5h It is an enzyme activity unit that collagen, which generates and is equivalent to the enzyme amount of the L-Leu of 1 μm of ol,.
The definition of the enzyme activity unit of neutral proteinase is: under conditions of pH 7.5 and 37 DEG C, hydrolyzing junket egg per minute The white enzyme amount for generating the Folin positive amino acid or peptide that are equivalent to 1 μm of ol tyrosine is an enzyme activity unit.
The definition of the enzyme activity unit of trypsin inhibitor is: can inhibit the vigor of a trypsase enzyme activity unit A referred to as inhibitor enzyme activity unit (U), under conditions of pH 7.5 and 25 DEG C, each second hydrolyzes the N- benzoyl-of 1 μm of ol L-arginine ethyl ester (BAEE) is a trypsase enzyme activity unit.
The definition of the enzyme activity unit of deoxyribonuclease is: under conditions of pH 8.0 and 37 DEG C, energy in 10 minutes Enzyme amount needed for the pBR322 Plasmid DNA of enough degradable 1 μ g is an enzyme activity unit.
It is provided by the invention separated from non-normal tissue single celled method include: by non-normal tissue's sample and digestion Liquid mixing is digested, and the digestive juice contains VIII Collagenase Type, neutral proteinase, trypsin inhibitor and deoxyribose Nuclease.
In the method, the ratio between VIII Collagenase Type and the enzyme activity unit of deoxyribonuclease is 100- 312.5:1, as 100:1,120:1,130:1,150:1,180:1,200:1,220:1,240:1,260:1,280:1,300:1, Arbitrary value between 310:1,312:1,312.5:1 or above-mentioned numerical value.
In the method, the ratio between neutral proteinase and the enzyme activity unit of deoxyribonuclease is 1-5:1, such as Arbitrary value between 1:1,1.5:1,2:1,2.5:1,3:1,3.5:1,4:1,4.5:1,5:1 or above-mentioned numerical value.
In the method, the ratio between trypsin inhibitor and the enzyme activity unit of deoxyribonuclease is 5000-25000:1, as 5000:1,8000:1,9000:1,10000:1,12000:1,15000:1,18000:1,20000:1, Arbitrary value between 22000:1,24000:1,25000:1 or above-mentioned numerical value.
Clostridiopetidase A is that unique one kind can degrade the protease of the natural collagen fibre with three strands of superhelixes, this Collagenous fibres are widely present in connective tissue.Clostridiopetidase A mainly by the fermented culture of clostridium histolyticum, is extracted, is refined And obtain, it can also extract and obtain from pig pancreas.In the present invention, the clostridiopetidase A is VIII Collagenase Type, for example, can be The Cat:C2139 of Sigma.
In the present invention, the specific type of neutral proteinase and deoxyribonuclease is not required particularly, Ke Yiwei The common various selections in this field.
Preferably, the neutral proteinase is Dispase II.For example, the Cat:4942078001 of Roche.
Preferably, the deoxyribonuclease is DNaseI.For example, the Cat:M0303S of NEB.
In the present invention, trypsin inhibitor can inhibit trypsase and chymotrypsin, prevent the active egg of other in pancreas The activation of white proenzyme and itself activation of trypsinogen, can choose trypsin inhibitor commonly used in the art.Example Such as, the Cat:T6522 of Sigma.
In the present invention, the digestive juice contains solvent.Relative to every milligram of VIII Collagenase Type, the content of the solvent Can be 0.1-12.5mL, preferably 0.2-3mL, as 0.2mL, 0.4mL, 0.5mL, 0.8mL, 1mL, 1.2mL, 1.3mL, Arbitrary value between 1.5mL, 2mL, 2.5mL or above-mentioned numerical value.
In the present invention, the solvent can be various common preservations or the reagent of dissolution enzyme preparation, it is preferable that described molten Agent is the phosphate buffer containing 4-10 volume % fetal calf serum.
In the present invention, the dosage of the digestive juice is not required particularly, as long as the sample can be submerged.It is excellent It is 1cm relative to volume in the case of choosing3Non-normal tissue's sample, the dosage of the digestive juice is 20-45mL, as 20mL, Arbitrary value between 25mL, 26mL, 27mL, 28mL, 30mL, 32mL, 35mL, 40mL, 45mL or above-mentioned numerical value.
In the present invention, in order to preferably be digested, the volume of non-normal tissue's sample is preferably 1-2cm × 1- 2cm × 0.5-2cm, such as 1.5cm × 1.5cm × 0.5cm.
In the present invention, the digestion can carry out under normal conditions.Preferably, the condition of the digestion includes that temperature is It is 35-38 DEG C, such as any between 35 DEG C, 36 DEG C, 36.5 DEG C, 36.8 DEG C, 37 DEG C, 37.2 DEG C, 37.5 DEG C, 38 DEG C or above-mentioned numerical value Value.
Preferably, the condition of the digestion further include the time be 5-80min, as 5min, 10min, 20min, 25min, 30min, 35min, 40min, 45min, 50min, 55min, 60min, 65min, 70min, 75min, 80min or above-mentioned numerical value it Between arbitrary value.
The digestion can carry out on shaking table, it is preferable that the condition of the digestion further comprises that vibration rate is 40- 60rpm/min。
In the present invention, it is adhered pockets of treatments of the sample in order to further speed up, it can be with shear sample and/or by suction pipe (such as Wu Junbushi suction pipe) blows and beats sample.It is filtered after a period of time can also be digested through cell sieve, then into indigested sample Digestive juice is added to continue to digest.That is, the mode of the digestion can be with are as follows: mix sample with first part digestive juice, shear Sample, and the sample after shearing is mixed with second part digestive juice, sample is blown and beaten, cell sieve is crossed, indigested sample is added Digestive juice continues to digest, and crosses cell sieve, and merges the filtrate for crossing cell sieve twice.It is 1cm relative to volume3Non-normal tissue Sample, the dosage of first part's digestive juice can be 400-1000 μ L.It is 1cm relative to volume3Non-normal tissue's sample, The dosage of two partial digested liquid can be 10-20mL.It is 1cm relative to volume3Non-normal tissue's sample, the digestive juice added Dosage can be 10-20mL.
In the present invention, in order to further promote the progress of digestion, the method also includes: before digestion, in tissue preserration Fiber, fat and the necrotic tissue of non-normal tissue's sample are removed in liquid.
Wherein, the dosage of the tissue preserration liquid is not required particularly, as long as the sample can be submerged.Institute Stating tissue preserration liquid can be conventional selection, for example, can be the serum-free cell containing fetal calf serum and protease inhibitors Freezing media.
In the present invention, the method also includes: postdigestive sample is contacted with erythrocyte cracked liquid to crack red thin Born of the same parents obtain the unicellular of separation after washing.Postdigestive sample be cell suspending liquid, be centrifuged and take precipitating, precipitate with it is red Cell pyrolysis liquid is contacted to remove red blood cell.The dosage of the erythrocyte cracked liquid can be conventional selection, for example, relative to body Product is 1cm3Non-normal tissue's sample, the dosage of the erythrocyte cracked liquid can be 3-8ml.Washing lotion used in washing It can be conventional selection, for example, can be the phosphate buffer containing 0.02-0.08 weight % bovine serum albumin.To described The dosage of washing lotion is not particularly limited, for example, being 1cm relative to volume3Non-normal tissue's sample, the dosage of the washing lotion It can be 3-8ml.
A kind of specific embodiment according to the present invention, the described method comprises the following steps:
1) it in tissue preserration liquid, is pruned with Sterile ophthalmic and cuts non-normal tissue's sample (especially pancreatic neoplasm sample) On fiber, fat and necrotic tissue etc.;
2) sterile PBS washing;
3) sample is put into sterile centrifugation tube, it (is 1cm relative to volume that first part's digestive juice, which is added,3It is improper Tissue sample, the dosage of first part's digestive juice can be 400-1000 μ L);
4) it is cut using Sterile ophthalmic and tissue is cut into clast (about 2 × 2 × 1mm3), it operates on ice, shear time is no more than 5 Minute;
5) tissue debris is transferred in sterile tube, second part digestive juice is added, be placed on shaking table and digested (relatively In volume be 1cm3Non-normal tissue's sample, the dosage of second part digestive juice can be 10-20mL);
6) pockets of tissue debris piping and druming will be adhered using Wu Junbushi suction pipe to mix;
7) tissue clastic state is observed after continuing digestion, if being still adhered agglomerating, repeatedly step 6) -7), if tissue debris Dispersion, then continue to digest, and total digestion time is no more than 30min;
8) digestion finishes, and stands after reusing Wu Junbushi suction pipe piping and druming tissue debris, collects supernatant and cross cell sieve, obtain Filtrate is placed on ice;
9) it (is 1cm relative to volume that indigested tissue, which adds digestive juice,3Non-normal tissue's sample, the digestion added The dosage of liquid can be 10-20mL), continue to digest, tissue debris is blown and beaten using Wu Junbushi suction pipe, together with digestive juice and tissue Clast crosses cell sieve, obtains filtrate;
10) merge the filtrate obtained twice, centrifugation;
11) abandon supernatant, be added erythrocyte cracked liquid softly blow and beat, be resuspended precipitating, be protected from light at room temperature split it is red, if there is cotton-shaped difficulty Molten object then crosses cell again and weeds out and remove;
12) re-suspension liquid is transferred in sterile centrifugation tube and is centrifuged;
13) supernatant is abandoned, first part's washing lotion is added and softly blows and beats resuspension precipitating, it is meticulous again if there is cotton-shaped indissoluble object Born of the same parents, which weed out, to be removed, and re-suspension liquid is transferred to new sterile centrifugation tube and continuously adds second part washing lotion (first part's washing lotion and the The volume ratio of two part washing lotions can be 1:4-5);
14) it is centrifuged;
15) step 13) is repeated;
16) it is centrifuged.
Another specific embodiment according to the present invention, the described method comprises the following steps:
1) it in tissue preserration liquid, is pruned with Sterile ophthalmic and cuts non-normal tissue's sample (especially position where tumour Pancreas) on fiber, fat and necrotic tissue etc.;
2) sterile PBS washing;
3) sample is put into sterile centrifugation tube, it (is 1cm relative to volume that first part's digestive juice, which is added,3It is improper Tissue sample, the dosage of first part's digestive juice can be 400-1000 μ L);
4) it is cut using Sterile ophthalmic and tissue is cut into clast (about 2 × 2 × 1mm3), it operates on ice, shear time is no more than 5 Minute;
5) tissue debris is transferred in sterile petri dish, it (is 1cm relative to volume that second part digestive juice, which is added,3's Non-normal tissue's sample, the dosage of second part digestive juice can be 5-20mL);
6) it is blown and beaten using Wu Junbushi suction pipe, collects supernatant and cross cell sieve, take filtrate, indigested tissue debris, which is added, to disappear Change liquid continue to digest in sterile petri dish, until tissue digestion completely or obtain satisfied normal tissue it is unicellular (relative to Volume is 1cm3Non-normal tissue's sample, the dosage for the digestive juice added every time can be 5-20mL);
7) filtrate obtained in step 6) is centrifuged;
8) abandon supernatant, be added lysate softly blow and beat, be resuspended precipitating, be protected from light at room temperature split it is red, if there is cotton-shaped indissoluble object, Cell is crossed again weed out remove;
9) re-suspension liquid is transferred in sterile centrifugation tube and is centrifuged;
10) supernatant is abandoned, first part's washing lotion is added and softly blows and beats resuspension precipitating, it is meticulous again if there is cotton-shaped indissoluble object Born of the same parents, which weed out, to be removed, and re-suspension liquid is transferred to new sterile centrifugation tube and continuously adds second part washing lotion (first part's washing lotion and the The volume ratio of two part washing lotions can be 1:4-5);
11) it is centrifuged;
12) step 10) is repeated;
13) it is centrifuged.
In the present invention, the method can also include using cell culture medium to digesting resulting unicellular cultivate. The cell culture medium can be the conventional medium for expanding cell, or the dimensional culture base containing growth factor, So that the single cells grown obtained is three-dimensional organoid model.
In the present invention, non-normal tissue's sample can be common abnormal tissue sample due to the factors such as lesion, It can be pancreatic samples, such as the tumor tissues in pancreas source.Method of the invention is particularly suitable for separate from pancreatic samples Unicellular, therefore, according to the preferred embodiment of the present invention, non-normal tissue's sample is that (pancreas is swollen for pancreatic neoplasm sample Tumor tissue) and/or tumour where position pancreas (pancreatic tissue).
The present invention will be described in detail by way of examples below.
Table 1
Table 2
Embodiment 1
The present embodiment is used to illustrate of the invention unicellular from normal pancreatic tissue (pancreas at position where tumour) separation Method, wherein used tissue preserration liquid, digestive juice, lysate and washing lotion are as shown in table 1, each in every liter of digestive juice The enzyme activity unit value and concentration of ingredient are as shown in table 2, and the preparation method of digestive juice are as follows: mixing VIII Collagenase Type, Dispase II and trypsin inhibitor dissolve mixing powder using solvent, add DNaseI mixing.
Sample is divided into five groups and is tested and (be shown in Table 3), specific steps are as follows:
1) in tissue preserration liquid, it is (normal that fiber, fat and necrotic tissue cut on sample etc. is pruned with Sterile ophthalmic Pancreatic tissue block size about 1.5 × 1.5 × 0.5cm3, color is yellow, and quality is medium partially soft, and surface is cut without black burnt necrosis, too many blood The visible clearly pancreas leaflet in face separates, and derives from pancreatic neoplasm patient, and operation cuts acquisition, patient's signed informed consent Book).
2) sterile PBS is washed 3 times.
3) sample is put into 5ml sterile EP tube (eppendorf), about 500 μ l of digestive juice is added.
4) it is cut using Sterile ophthalmic and tissue is cut into clast (about 2 × 2 × 1mm3), it operates on ice, shear time is no more than 5 Minute.
5) tissue debris is transferred in 10cm sterile petri dish, 10ml digestive juice is added, be placed in 37 DEG C of incubator digestion.
6) it is mixed once every 5min using the piping and druming of Wu Junbushi suction pipe, and is seen under 10 × 20,10 × 40 power microscopes Examine cell dissociation situation.There is individual cells suspension in visible digestive juice under the microscope when first 10min, by digestive juice It is collected into sterile 50ml centrifuge tube together with tissue debris, is stood after soft piping and druming, collect supernatant and cross 40 μm of cell sieve (cell Strainer), filtrate is taken.Indigested tissue debris adds digestive juice 10ml and continues to digest in 10cm sterile petri dish, directly It completely or obtains that satisfied pancreas normal tissue is unicellular (altogether continue 50min) to tissue digestion, first 10min is collected Filtrate is given it up, and because it contains more impurity, separates unicellular difficulty.The filtrate that later every 10min digests can be distinguished It retains, carries out aftermentioned operating procedure respectively, finally choose motility rate, the optimal single cell suspension sample of cell quantity.
7) filtrate 800g obtained in step 6) is centrifuged 4min (using horizontal rotor).
8) supernatant is abandoned, 5ml lysate is added and softly blows and beats, precipitating is resuspended, is protected from light splits red 5min (if there is cotton-shaped difficulty at room temperature Molten object then crosses 40 μm of cell sieve removals again).
9) re-suspension liquid is transferred in sterile 15ml centrifuge tube and is centrifuged, centrifugal force: 800g, time: 4min.
10) supernatant is abandoned, addition 1ml washing lotion softly blows and beats resuspension precipitating and (if there is cotton-shaped indissoluble object, crosses 40 μm of cells again Weed out and remove), re-suspension liquid is transferred to a new sterile 15ml centrifuge tube and continuously adds 5ml washing lotion.
11) 600g is centrifuged 5min.
12) step 10) is repeated.
13) 400g is centrifuged 6min.
14) supernatant is abandoned, precipitating is resuspended in appropriate washing lotion, and (precipitating of covering 15ml centrifugation bottom of the tube, uses 100 μ l washing lotion weights It is outstanding), take isometric cell and trypan blue to mix, microscopy cellular morphology, motility rate, impurity situation etc., cell counter (life Cell countess) detection Cell viability (living cells quantity accounts for the percentage of total number of cells in=every ml product) is (every with concentration Total number of cells in ml product, including dead cell), as a result as shown in Fig. 1-5 and table 3.
In Fig. 1-5, upper figure is the result figure for observing digestion effect after digesting under ordinary optical microscope (40 ×), the following figure For the result figure for observing Cell viability after further diluting under ordinary optical microscope (40 ×).
Table 3
From Fig. 1 and table 3 as can be seen that can effectively be separated from normal tissue using method of the invention it is unicellular, Basic soilless sticking, Cell viability is 85% or more.
From Fig. 2, Fig. 3 and table 3 as can be seen that if the ratio in digestive juice between each component is not in the scope of the present invention Interior, cell, which exists, after digestion reunites, and Cell viability is relatively low.
From Fig. 4 and table 3 as can be seen that can be obtained using VIII Collagenase Type more significantly more than other types of clostridiopetidase A Unicellular and Cell viability it is also higher.
From Fig. 5 and table 3 as can be seen that being only used cooperatively VIII Collagenase Type, neutral proteinase, trypsin inhibitor Single cells population (reuniting few) and Cell viability can be effectively improved with deoxyribonuclease, four kinds of ingredients are indispensable, Collaboration plays a role.
Embodiment 2
The present embodiment is used to illustrate of the invention from the single celled method of pancreas source tumor tissues separation, wherein is made Tissue preserration liquid, digestive juice, lysate and washing lotion are as shown in table 1, each in every liter of digestive juice (preparation method is with embodiment 1) The enzyme activity unit value and concentration of a ingredient are as shown in the I-1 of table 2.
1) it in tissue preserration liquid, is pruned with Sterile ophthalmic and cuts pancreatic neoplasm sample (1.5 × 1.5 × 0.5cm3, operation Cut acquisition, patient's signed informed consent form) on fiber, fat and necrotic tissue etc..
2) sterile PBS is washed 3 times.
3) sample is put into 5mL sterile EP tube (eppendorf), about 500 μ l of digestive juice is added.
4) it is cut using Sterile ophthalmic and tissue is cut into clast (about 2 × 2 × 1mm3), it operates on ice, shear time is no more than 5 Minute.
5) tissue debris is transferred in 50ml sterile tube, 15ml digestive juice is added, be placed in 37 DEG C, 50rmp/min shakes It is digested on bed.
6) pockets of tissue debris piping and druming will be adhered using Wu Junbushi suction pipe after 5min to mix.
7) continue to observe tissue clastic state after digesting 5min, if being still adhered agglomerating, repeatedly step 6) -7), if tissue Clast dispersion then continues to digest 20min, and total digestion time is no more than 30min.
8) digestion finishes, and stands 3min after reusing Wu Junbushi suction pipe piping and druming tissue debris, collects supernatant and cross 40 μm Cell sieve (cell strainer), obtains filtrate and is placed on ice.
9) indigested tissue adds 15ml digestive juice, continues after digesting 20min, blows and beats tissue using Wu Junbushi suction pipe Clast crosses 40 μm of cell sieves together with digestive juice and tissue debris, obtains filtrate.
10) merge the filtrate obtained twice, 800g is centrifuged 4min (using horizontal rotor).
11) supernatant is abandoned, 5ml lysate is added and softly blows and beats, precipitating is resuspended, is protected from light splits red 5min (if having cotton-shaped at room temperature Indissoluble object then crosses 40 μm of cell sieve removals again).
12) re-suspension liquid is transferred in sterile 15ml centrifuge tube and is centrifuged, centrifugal force: 800g, time: 4min.
13) supernatant is abandoned, addition 1ml washing lotion softly blows and beats resuspension precipitating and (if there is cotton-shaped indissoluble object, crosses 40 μm of cells again Weed out and remove), re-suspension liquid is transferred to a new sterile 15ml centrifuge tube and continuously adds 5ml washing lotion.
14) 600g is centrifuged 5min.
15) step 13) is repeated.
16) 400g is centrifuged 6min.
17) supernatant is abandoned, precipitating is resuspended in appropriate washing lotion, and (precipitating of covering 15ml centrifugation bottom of the tube, uses 100 μ l washing lotion weights It is outstanding), take isometric cell and trypan blue to mix, microscopy cellular morphology, motility rate, impurity situation etc., cell counter (life Cell countess) Cell viability and concentration are detected, it is as a result similar to Example 1, it can be effectively using method of the invention Separated from tumor tissues unicellular, basic soilless sticking, Cell viability is 80% or more;And if in digestive juice each group point it Between ratio cell exists not within the scope of the invention, after digestion reunites, Cell viability is relatively low;And use VIII Collagen Type VI It is also higher that enzyme can obtain the unicellular and Cell viability more significantly more than other types of clostridiopetidase A.In addition, lacking one kind In the case where ingredient, single cells population and Cell viability are undesirable, further illustrate that four kinds of ingredients are indispensable, and collaboration plays Effect.
The preferred embodiment of the present invention has been described above in detail, and still, the present invention is not limited thereto.In skill of the invention In art conception range, can with various simple variants of the technical solution of the present invention are made, including each technical characteristic with it is any its Its suitable method is combined, and it should also be regarded as the disclosure of the present invention for these simple variants and combination, is belonged to Protection scope of the present invention.

Claims (10)

1. one kind separates single celled method from non-normal tissue, which is characterized in that this method comprises: by non-normal tissue's sample Product are mixed with digestive juice to be digested, the digestive juice contain VIII Collagenase Type, neutral proteinase, trypsin inhibitor and Deoxyribonuclease, wherein the VIII Collagenase Type, neutral proteinase, trypsin inhibitor and DNA Ratio between the enzyme activity unit of enzyme is 100-312.5:1-5:5000-25000:1.
2. according to the method described in claim 1, wherein, the neutral proteinase is Dispase II;
And/or the deoxyribonuclease is DNaseI.
3. method according to claim 1 or 2, wherein relative to every milligram of VIII Collagenase Type, in the digestive juice Solvent content be 0.1-12.5mL.
4. according to the method described in claim 3, wherein, the solvent is slow for the phosphate containing 4-10 volume % fetal calf serum Fliud flushing.
5. according to the method described in claim 1, being 1cm relative to volume wherein3Non-normal tissue's sample, the digestive juice Dosage be 20-45mL.
6. method according to claim 1 or 5, wherein the volume of non-normal tissue's sample is 1-2cm × 1-2cm ×0.5-2cm。
7. according to the method described in claim 1, wherein, the condition of the digestion includes: that temperature is 35-38 DEG C, time 5- 80min, vibration rate 40-60rpm/min.
8. according to the method described in claim 1, wherein, the method also includes: before digestion, removed in tissue preserration liquid Fiber, fat and the necrotic tissue of non-normal tissue's sample.
9. according to the method described in claim 8, wherein, the tissue preserration liquid is to contain fetal calf serum and protease inhibitors Serum-free cell freezing media.
10. according to claim 1, method described in 8 or 9, wherein the method also includes: by postdigestive sample and red thin The contact of cellular lysate liquid obtains the unicellular of separation to splitting erythrocyte after washing.
CN201811594140.0A 2018-12-25 2018-12-25 Method for isolating single cells from abnormal tissue Active CN109609439B (en)

Priority Applications (1)

Application Number Priority Date Filing Date Title
CN201811594140.0A CN109609439B (en) 2018-12-25 2018-12-25 Method for isolating single cells from abnormal tissue

Applications Claiming Priority (1)

Application Number Priority Date Filing Date Title
CN201811594140.0A CN109609439B (en) 2018-12-25 2018-12-25 Method for isolating single cells from abnormal tissue

Publications (2)

Publication Number Publication Date
CN109609439A true CN109609439A (en) 2019-04-12
CN109609439B CN109609439B (en) 2020-11-06

Family

ID=66012345

Family Applications (1)

Application Number Title Priority Date Filing Date
CN201811594140.0A Active CN109609439B (en) 2018-12-25 2018-12-25 Method for isolating single cells from abnormal tissue

Country Status (1)

Country Link
CN (1) CN109609439B (en)

Cited By (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN110257318A (en) * 2019-05-27 2019-09-20 上海长海医院 A kind of preparation method of chronic pancreatitis mice pancreatic single cell suspension
CN112662614A (en) * 2021-01-12 2021-04-16 四川大学华西医院 Kit and method for preparing pancreatitis tissue single cell suspension

Citations (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN202465674U (en) * 2012-03-07 2012-10-03 上海安集协康生物技术有限公司 Stem cell extraction device
CN105176917A (en) * 2015-11-02 2015-12-23 广州赛莱拉干细胞科技股份有限公司 Culture medium and application thereof, and keratinocyte culture method
CN107119008A (en) * 2017-05-05 2017-09-01 中南大学 A kind of young porcine islet isolation method and separation digestive juice
CN108103013A (en) * 2018-01-26 2018-06-01 河北医科大学第四医院 The enzyme digestion original cuiture and identification method of a kind of gastric and esophageal engaging portion smooth muscle cell

Patent Citations (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN202465674U (en) * 2012-03-07 2012-10-03 上海安集协康生物技术有限公司 Stem cell extraction device
CN105176917A (en) * 2015-11-02 2015-12-23 广州赛莱拉干细胞科技股份有限公司 Culture medium and application thereof, and keratinocyte culture method
CN107119008A (en) * 2017-05-05 2017-09-01 中南大学 A kind of young porcine islet isolation method and separation digestive juice
CN108103013A (en) * 2018-01-26 2018-06-01 河北医科大学第四医院 The enzyme digestion original cuiture and identification method of a kind of gastric and esophageal engaging portion smooth muscle cell

Non-Patent Citations (3)

* Cited by examiner, † Cited by third party
Title
PEAKMAN MARK ET AL.: "development of techniques for obtaining monodispersed human islet cells", 《TRANPLANTATION》 *
李丹: "成体小鼠胰腺单细胞的离体分离、分析及培养", 《中国优秀硕士学位论文全文数据库 医药卫生科技辑》 *
李杨等: "联合应用乌斯他丁和DNA酶提高分离胰岛的效果的实验研究", 《2012中国器官移植大会论文汇编》 *

Cited By (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN110257318A (en) * 2019-05-27 2019-09-20 上海长海医院 A kind of preparation method of chronic pancreatitis mice pancreatic single cell suspension
CN110257318B (en) * 2019-05-27 2023-05-30 上海长海医院 Preparation method of pancreatic single cell suspension of chronic pancreatitis mice
CN112662614A (en) * 2021-01-12 2021-04-16 四川大学华西医院 Kit and method for preparing pancreatitis tissue single cell suspension
CN112662614B (en) * 2021-01-12 2023-09-08 四川大学华西医院 Kit and method for preparing pancreatitis tissue single-cell suspension

Also Published As

Publication number Publication date
CN109609439B (en) 2020-11-06

Similar Documents

Publication Publication Date Title
CN109666625A (en) Single celled method is separated from tissue
CN109694845A (en) For separating single celled kit and its application
CA2948952C (en) Process and device for isolating cells from biological tissue
EP1266959B1 (en) Devices and method for cell harvesting
CN109666644A (en) Single celled method is separated from tumor sample
CN112708610B (en) Mixed enzyme for skin tissue dissociation, preparation method thereof, dissociation kit and dissociation method
JPH02504222A (en) Methods for isolating subtype cell clusters from organs
US10329533B2 (en) Regenerative cell and adipose-derived stem cell processing system and method
CN112662614B (en) Kit and method for preparing pancreatitis tissue single-cell suspension
CN101984049A (en) Method for separating mesenchymal stem cells from dispose tissues
CN109609439A (en) Single celled method is separated from non-normal tissue
CN109097320A (en) A kind of sheep lamb cud epithelial cell cultural method
CN101848718A (en) The cell composition that is used for tissue regeneration
CN109628434A (en) It is single celled containing enzymatic compositions and its preparation method and application for separating
CN109536449A (en) Single celled method is separated from abnormal structure
CN109666626A (en) Single celled method is separated from sample
CN109694846A (en) Kit and its application containing trypsin inhibitor
CN107227295A (en) Come off separation and the in-vitro multiplication method of deciduous teeth stem cell
CN109628394A (en) A method of extraction umbilical cord mesenchymal stem cells of the grinding in conjunction with mixed enzyme
CN109735515A (en) Composition and its preparation method and application containing clostridiopetidase A
CN109609438A (en) Single celled method is separated from non-tumor sample
CN109666624A (en) Kit and its application containing clostridiopetidase A
CN109762796A (en) Composition and its preparation method and application containing trypsin inhibitor
CN112175902B (en) Separation method of adipose-derived stem cells
CN106676063A (en) Separate culture method for human amniotic mesenchymal stem cells

Legal Events

Date Code Title Description
PB01 Publication
PB01 Publication
SE01 Entry into force of request for substantive examination
SE01 Entry into force of request for substantive examination
GR01 Patent grant
GR01 Patent grant