国产一卡2卡三卡4卡麻豆_了解最新日韩草逼视频_h片在线播放一区_国产激情影视在线_好了av四色综合无码久久_欧美黑白双插OOR720P_日本精品中文字幕在线_秋霞午夜手机影院_亚洲国产一区二区3da毛片_欧美杂交深喉video中文字幕

官方微信|手機版

產品展廳

產品求購企業資訊會展

發布詢價單

化工儀器網>產品展廳>試劑標物>生化試劑>培養基> 類器官Gastric Cancer Organoid Kit

分享
舉報 評價

類器官Gastric Cancer Organoid Kit

參考價 5158.00-11880.00
具體成交價以合同協議為準
規格
100ml5158.00元100 ml 可售
500ml11880.00元500 ml 可售

聯系方式:林明查看聯系方式

聯系我們時請說明是化工儀器網上看到的信息,謝謝!


       

普邁精醫科技(北京)有限公司(PRECISION MEDICINE TECHNOLOGY(Beijing)Co.LTDEVOQUA德國懿華在中國的合作伙伴,為實驗室客戶提供專業的科研檢測設備解決方案。

我們了解科學儀器在全球的應用,匯集于專業的解決方案,傳遞給國內頂級科研及檢測人員,輔助我們的客戶取得事業進步和成功。

我們提供的專業解決方案有:

實驗室純水及超純水供給解決方案:可根據客戶需求,提供1.2-14/分鐘的超純水,10-1000/小時的純水設備及設計方案,并提供全部相關耗材,EDI去離子模塊。

生物樣本庫解決方案:樣本庫前期設計、各功能區規劃到樣本前后處理設備、樣本凍存耗材、樣本凍存設備,再到樣本自動化工作站、自動化樣本庫、樣本庫管理軟件,為客戶提供一站式樣本存儲解決方案。

細胞培養解決方案:該方案涵蓋組織提取,研磨消解,培養分選,生化分析,分離富集,凍存轉運各環節的儀器設備及耗材,并提供相關檢測服務及科研服務。

細胞囊泡及外泌體EXOSOME解決方案:該方案涵蓋細胞囊泡及外泌體EXOSOME的分離提取,鑒定鑒別,測序分析及后續應用。我們為客戶提供相關環節專業儀器,試劑盒,耗材,并提供相關檢測服務及科研服務。

分子生物學解決方案:該方案包含基因表達,分子克隆,蛋白表達,核酸檢測等各分子生物學研究領域所需要的設備及耗材,并提供流程自動化方案和技術服務。

醫療科研解決方案:普邁精醫針對醫療科研行業,根據醫療科研人員的實際需求,整合以上多個解決方案,并和眾多優秀廠家合作,開發傳統科學儀器在醫療上的創新型應用,為客戶提供多方位的醫療科研和醫療檢驗儀器,耗材,技術服務保障。

 

 

 

 

 

 

 

通用實驗室設備,分子生物學設備,顯微鏡,成像設備,科研用耗材

供貨周期 現貨

類器官Gastric Cancer Organoid Kit


類器官(Organoids)是指將成體干細胞或多能干細胞在體外三維培養形成的具有一定空間結構的組織類似物。類器官在組織結構、細胞類型、自我更新能力和功能等方面與來源組織高度一致,從而在發育生物學、疾病造模、精準醫學、藥物研發、基因和細胞療法、感染和免疫以及再生醫學等生物醫學的多個領域展現出*的優勢。

產品介紹
Product Description:
bioGenousTM Gastric Cancer Organoid Kit is a chemically defined cell culture medium for the establishment and maintenance of human gastric cancer organoid s. Patient-derived cancer organoids recapitulate the genomic and pathological features of original tumors and therefore hold great promise for medical research and precision medicine.


技術參數Product Information:

ComponentComponent Cat#VolumeStorage & Stability
bioGenousTM Gastric Cancer Organoid Basal MediumK2179-GC-A100/A500100mL/500mL412 months
bioGenousTM Gastric Cancer Organoid Supplement B (50x)K2179-GC-B100/B5002mL/10mL-20, avoid repeated freeze-thaw cycles, 12 months
bioGenousTM Gastric Cancer Organoid Supplement C (250x)K2179-GC-C100/C5000.4mL/2mL-20, avoid repeated freeze-thaw cycles, 12 months

Preparation of Gastric Cancer Organoid Complete Medium
Use a sterile technique to prepare the gastric cancer organoid complete medium. The following example is for preparing 10mL complete medium. If preparing other volumes, adjust accordingly.
1.      Thaw Gastric Cancer Organoid Supplement B(50x) and Gastric Cancer Organoid Supplement C(250x) on ice. Mix thoroughly.
NOTE: Once thawed, use immediately or aliquot and store at -20°C for not more than 10 months. After thawing the aliquots, use immediately. Do not re-freeze.
2.      Add 200μL Gastric Cancer Organoid Supplement B(50x) and 40μL Gastric Cancer Organoid Supplement C(250x) to 9.76mL Gastric Cancer Organoid Basal Medium. Mix thoroughly.
NOTE: If not used immediately, store the complete medium at 2-8°C for not more than 2 weeks. The Gastric Cancer Organoid Supplement B contains fungicide and antibiotics (50x).
Protocol for Establishment of Patient-Derived Gastric Cancer Organoids
CAUTION Studies involving primary human tissue material must follow all relevant institutional and government regulations. Informed consent must be obtained from all subjects before the collection of the primary human tissue material.
Establishment of Organoids from Primary Tissue
1.      Collect primary human gastric cancer tissue pieces in ice-cold Primary Tissue Storage Solution (K601005) with conical tubes. Keep tissue samples at 4°C until the start of the isolation.
2.      Assess whether the obtained tissue pieces consist purely of epithelium. If fat or muscle tissues are present, remove these non-epithelial components as much as possible using surgical scissors or scalpels and forceps under a dissection microscope. If no fat or muscle tissues are present, continue to the next step immediately.
3.      Rinse the tissue with Cancer Organoid Basal Medium (B213152) or DPBS twice.
4.      Mince the tissue into small fragments of 1-3 mm3 in a cell culture dish using surgical scissors or scalpels.
5.      Digest the tissue fragments with 10mL of Tumor Tissue Digestion Solution (K601003) in a 15mL conical tube at 37°C, with variable incubation times ranging from 30 min to 1 h. Carefully monitor the digestion process, mixing the content of the tube every 5-10 min by shaking vigorously or pipetting the mixture up and down. The digestion process could be finished when most of tissue fragments are able to pass through the 1mL pipette tips.
6.      Add FBS to the tissue digestion mixture to a final concentration of 2%, and filter using a 100 μm cell strainer.
7.      Collect and centrifuge the filtered cells at 250g for 3 min at 4 °C. In case of a visible red pellet, aspirate the supernatant, and resuspend the pellet using 2mL of Red Blood Cell Lysis Solution (E238010) to lyse the erythrocytes at room temperature for 1 min and centrifuge at 250g for 3 min at 4°C.
8.      Aspirate the supernatant and resuspend the pellet in Cancer Organoid Basal Medium, centrifuge at 250g for 3 min at 4°C, repeat this step once more time.
9.      Aspirate the supernatant and resuspend the pellet in Matrigel. The Matrigel should be kept on ice to prevent it from solidifying. Perform the process as quickly as possible. The amount of Matrigel used depends on the size of the pellet. Approximately 10,000 cells should be plated in 25 μL of Matrigel.
CRITICAL: Do not overly dilute the Matrigel (Matrigel should be >70% (Matrigel vol/Total vol)), as this may inhibit the proper formation of the solid droplets.
10.   Plate the Matrigel containing organoids at the bottom of 24-well cell culture plates in droplets of ~30 μL each around the center of the well..
CRITICAL: Once the organoids are resuspended in Matrigel, proceed with plating as quickly as possible, as the Matrigel may solidify in the tube or pipette tip. Do not let the Matrigel touch the wall of wells.
11.   Place the culture plate into a humidified incubator at 37 °C and 5% (vol/vol) CO2 for 15-25 min to let the Matrigel solidify.
12.   Prepare the required amount of gastric cancer organoid complete medium.
13.   Once the Matrigel droplets have solidified (15-25 min), open the plate and carefully add 500 μL of organoid complete medium to each well.
CRITICAL: Do not add the medium directly on top of the Matrigel droplets, as this might disrupt the droplets.
14.   Place the culture plate in a humidified incubator at 37 °C and 5% (vol/vol) CO2.
15.   Change the medium every 3-4 d by carefully aspirating the medium from the wells and replacing it with a fresh, pre-warmed organoid complete medium.
16.   Closely monitor the organoid formation. Ideally, patient-derived gastric cancer organoids should be passaged for the first time between 7 and 10 d after the initial plating.
Splitting and Passaging of Organoids
17.   Pipette up and down to disrupt the Matrigel and transfer the organoid suspension to a 1.5 mL conical tube.
18.   Pipette the organoid suspension up and down to mix thoroughly by pipetting against the bottom of the tube to create pressure, which will aid the removal of Matrigel.
19.   Centrifuge organoids at 250g for 3 min at room temperature.
20.   Aspirate the supernatant and split organoids using either Organoid Dissociation Solution (E238001) or by mechanical disruption. For Organoid Dissociation Solution-based cell dissociation, resuspend the pellet in 0.2 mL of Organoid Dissociation Solution, pipette up and down and incubate at 37 °C until organoids fall apart. Pipette up and down with a filter tip for ≥8 times every 2 min to aid in the disruption of the organoids. Closely monitor the digestion to keep the incubation time in the Organoid Dissociation Solution to a minimum. In case of mechanical disruption, resuspend the pellet in 1.5 mL of Cancer Organoid Basal Medium. Carefully pipette the organoid suspension up and down 30 times by pipetting against the bottom of the tube to create pressure, which will aid organoid disruption.
CRITICAL: Do not dissociate in Organoid Dissociation Solution for >5 min, as this may result in poor organoid outgrowth or even loss of the culture. As a rule of thumb, digestion is complete if a mixture of small lumps of cells (consisting of 10–50 cells) can be observed.
21.   After shearing is complete, wash once by topping up with 1 mL of Cancer Organoid Basal Medium, and centrifuge at 250g for 3 min at room temperature.
22.   Aspirate the supernatant and resuspend the organoid pellet in 70% (vol/vol) Matrigel, and plate organoids in droplets at the bottom of a culture plate as described in Steps 10. After plating is complete, transfer the plate into a humidified incubator at 37 °C and 5% (vol/vol) CO2 for 15–25 min.
23.   Pre-warm gastric cancer organoid complete medium at 37 °C.
24.   After the Matrigel droplets have solidified (15–25 min), carefully pipette pre-warmed medium into the wells.
25.   Place culture plates in a humidified incubator at 37 °C and 5% (vol/vol) CO2 until the organoids are needed for further experiments.



類器官Gastric Cancer Organoid Kit



化工儀器網

采購商登錄
記住賬號    找回密碼
沒有賬號?免費注冊

提示

×

*您想獲取產品的資料:

以上可多選,勾選其他,可自行輸入要求

個人信息:

溫馨提示

該企業已關閉在線交流功能

主站蜘蛛池模板: 社旗县| 望城县| 城口县| 建昌县| 金湖县| 平遥县| 东乡族自治县| 安庆市| 宁夏| 云和县| 奈曼旗| 岚皋县| 泾阳县| 柘荣县| 顺义区| 舟曲县| 句容市| 庆安县| 扬州市| 高邮市| 和平区| 泰宁县| 九龙坡区| 景洪市| 观塘区| 汕尾市| 高尔夫| 井冈山市| 阿鲁科尔沁旗| 梧州市| 年辖:市辖区| 思茅市| 望江县| 秭归县| 景泰县| 新邵县| 南皮县| 大埔县| 射阳县| 博野县| 万年县|