槲皮苷对照品

7种混合阴离子对照品 I, 50 mL

6种阳离子混合对照品-II, 50 mL

NanoTemper 推出 NT.115 对照试剂盒（红色），可用于检测配备有 Nano-GREEN/RED、Nano-BLUE/RED 或 Pico-RED 探测器的 MO 系列仪器的性能、或对第一次操作该系统的新用户进行培训。

NanoTemper 推出 NT.115 对照试剂盒（绿色），可用于检测配备有 Nano-GREEN/RED、Nano-BLUE/GREEN 探测器的 MO 系列仪器的性能，或对第一次操作该系统的新用户进行培训。

SureGuide gRNA 对照试剂盒为 CRISPR 研究提供对照 gRNA 和对照 DNA 靶标。对照 gRNA 为 gRNA 制备的质量评估提供了参比。对照 DNA 靶标用于测量 CRISPR/Cas 实验中的酶切效率。 包含这些对照以获得安捷伦用于体外 CRISPR/Cas 研究的一体化解决方案的所有优势。特征明确的对照材料可监测 CRISPR/Cas 实验每个步骤的情况。 知晓您的实验何时成功并尽早纠正任何问题。在进行进一步的实验之前，对照 gRNA 有助于评估 gRNA 制备的质量，在制备的 gRNA 不适用时避免浪费时间和精力，适用时可进一步增加您对实验的信心。对照 DNA 靶标用于确定 CRISPR/Cas 实验中的 DNA 酶切效率，以确认实验结果的有效性。根据您的需求量身定制。联系我们 返回页首/SpecificationsSectionPageletTemplate --/TechnologySectionPageletTemplate --/SideBySideSectionPageletTemplate --var sections = ' script=""/ApplicationsSectionPageletTemplate --var sections = '' /LiteratureSectionPageletTemplate --libraryContentType = 'LibraryContent_C' window.literatureTagged = '[1405071398204, 1404948115389, 1404948113181]' window.regulatoryFlag='true' document.getElementById('product-details').className = "" document.getElementById('product-details').className = "heading" console.log("document.getElementById('product-details').className is"+document.getElementById('product-details').className) 联系我们 返回页首/SpecificationsSectionPageletTemplate --/TechnologySectionPageletTemplate --/SideBySideSectionPageletTemplate --var sections = ' script=""资料库联系我们 返回页首/SpecificationsSectionPageletTemplate --/TechnologySectionPageletTemplate --/SideBySideSectionPageletTemplate --var sections = ' script=""数据表联系我们 返回页首/SpecificationsSectionPageletTemplate --/TechnologySectionPageletTemplate --/SideBySideSectionPageletTemplate --var sections = ' script="" langString : zh -- langString : zh --联系我们 返回页首/SpecificationsSectionPageletTemplate --/TechnologySectionPageletTemplate --/SideBySideSectionPageletTemplate --var sections = ' script=""联系我们 返回页首/SpecificationsSectionPageletTemplate --/TechnologySectionPageletTemplate --/SideBySideSectionPageletTemplate --var sections = ' script=""联系我们 返回页首/SpecificationsSectionPageletTemplate --/TechnologySectionPageletTemplate --/SideBySideSectionPageletTemplate --var sections = ' script=""联系我们 返回页首/SpecificationsSectionPageletTemplate --/TechnologySectionPageletTemplate --/SideBySideSectionPageletTemplate --var sections = ' script="" SureGuide Cas9 Programmable Nuclease Kit_5991-5149EN The CRISPR/Cas in vitro system is a complete and ready-to-use kit for performing unrestricted in vitro cloning of large DNA fragments without the limitation of common RE's 数据表 English 2014 年 9 月 2 日 748.47 KB PDF var x=document.querySelector('nav.pdp-nav').children for(var i=0 i langString : zh -- langString : zh -- SureGuide gRNA Synthesis Kit Datasheet 5991-5148EN The SureGuide gRNA synthesis kit is designed for the rapid and simple preparation of gRNAs to be used in conjunction with the SureGuide Cas9 system (part no 5190-7714). 数据表 English 2014 年 8 月 29 日 744.08 KB PDF var x=document.querySelector('nav.pdp-nav').children for(var i=0 i宣传单页 返回页首/SupportSectionPageletTemplate --window.supportTagged = 'null' window.regulatoryFlag = 'true' window.supportFeatured = '' window.libSupportTagged = '1404948873769' 技术支持用户手册document.getElementById('product-details').className = "" document.getElementById('product-details').className = "heading" var x=document.querySelector('nav.pdp-nav').children for(var i=0 i langString : zh -- langString : zh -- SureGuide gRNA Synthesis Kit Protocol SureGuide gRNA Synthesis Kit Protocol 用户手册 English 2015 年 4 月 7 日 688.02 KB PDF var x=document.querySelector('nav.pdp-nav').children for(var i=0 ivar x=document.querySelector('nav.pdp-nav').children for(var i=0 i 返回页首 /ReferencesSectionPageletTemplate --/SelectionToolsSectionPageletTemplate --document.getElementById('product-details').className = "" document.getElementById('product-details').className = "heading" 工具 SureVector 工具 创建您的图谱var x=document.querySelector('nav.pdp-nav').children for(var i=0 idocument.querySelector('.selectiontools').style.display= "block" 返回页首 /BenefitsSectionPageletTemplate --/TestimonialSectionPageletTemplate --/VideosSectionPageletTemplate --window.videoJSONURL = '/cs/ContentServer?d=&pagename=Agilent/Util/GetAssociatedAssets&assetId=1405155910678&assetType=Products_C&assetDimension=zh_CN&taggingBased=false&attributeName=prod_video&jsonVariable=relatedVideos®ulatoryFlag=true&locale=zh_CN¤tUrlLocale=zh-cn&countryCode=CN&displaySeeAll=false&assocList=[1405106787461]&assocType=MultimediaST_C' window.videoJSONMaxCount = 15 if(null!=document.querySelector('.videos')){document.querySelector('.videos').style.display= "block" }视频 用于生成出色的 sgRNA 文库的 CRISPer 指南 1:03:21 1 - 6 of 28 Results 返回顶部 /TrainingEventsSectionPageletTemplate --document.getElementById('product-details').className = "" document.getElementById('product-details').className = "heading" 培训与活动 Synthetic Biology: ... Swing by our booth from June 22-26, 2020 during the SEED conference at the Hyatt Regency, San Francisco. Learn everything there is to know on the newest advancements in synthetic biology. Come and discuss your CRISPR needs with our experts!网络研讨会/培训var x=document.querySelector('nav.pdp-nav').children for(var i=0 i TIDES: ... From May 11th to 14th 2020, you can find us at our booth during TIDES at the Hynes Convention Center, Boston. Looking for some expert advice to conduct successful CRISPR and oligo-experiments in your lab? Come talk to us!网络研讨会/培训var x=document.querySelector('nav.pdp-nav').children for(var i=0 i 6th Precision CRISPR ... Will you be there? Say hi to our CRISPR experts at our booth during the 6th Precision CRISPR Genome Editing Conference in Boston in May 2020. More details will follow!网络研讨会/培训var x=document.querySelector('nav.pdp-nav').children for(var i=0 i查看全部 返回页首/NewsSectionPageletTemplate --/ServicesSectionPageletTemplate --/OfficesSectionPageletTemplate --/RelatedProductsSectionPageletTemplate --window.applicationURL = '/cs/ContentServer?d=&pagename=Agilent/Util/GetRelatedAssets&taggingBased=false&assetId=1405155910678&assetType=Products_C&assetDimension=zh_CN¤tUrlLocale=zh-cn&countryCode=CN®ulatoryFlag=true&assocList=[PRDT_228332, PRDT_228331, PRDT_228324, PRDT_228323]' returnToTopText='Return to top' 相关产品 SureVector 文库克隆试剂盒 SureVector 文库克隆试剂盒包含从寡核苷酸混合物中克隆 ...类别: CRISPR 文库克隆试剂盒 SureGuide gRNA ... 从您的 DNA 模板可靠且方便地生成可直接用于 CRISPR/Cas ...类别: CRISPR gRNA 合成与对照试剂盒 SureGuide 定制已扩增文库 超高质量的 CRISPR 定制已扩增和混合 gRNA 文库类别: CRISPR 文库 SureGuide Cas9 ... 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SA990702 E10152 钨酐，颗粒状 25 g 天津欧捷科技有限公司---进口元素分析耗材供应商 保证质量天津欧捷科技是一家高科技企业，公司集贸易、科研、服务一体化。公司从精密仪器设备及配件、耗材、试剂、标准对照品、实验室常用耗材的销售，到仪器调试、维护、样品的分析测试。 实验室耗材 元素分析耗材 色谱分析耗材 质谱耗材样品容器 Labco顶空进样瓶 色谱瓶 石英棉 石英燃烧管 进样隔垫 催化剂 标准品 试剂 玻璃碳产品 仪器配件这些耗材可用在Thermo、Elementar、Agilent、Analytikjena、Sercon、Shimadzu、leco、Varian、Perkin Elmer、waters 、Euro Vector等仪器。

石墨赶酸器、石墨赶酸电热板一、产品介绍石墨赶酸器又称赶酸板、样品处理器、赶酸仪、消解器。适用于食品、疾控、农科院、医药、农业、林业、环保、化工、生化等行业以及高等院校、科研部门对微波消解、高压消解的后期赶酸,是原子吸收、原子荧光、ICP- AES、AA、ICP- MS等分析仪器的理想配套产品。石墨赶酸器参数型 号ZH控温范围室温-260℃控温精度±0.1℃，高温度差3-5℃加热材质优质石墨+特氟龙防腐涂层样品孔数20、25、30、40、42、48孔等（可根据客户要求加工定制）控显方式PID控温数显电 源220v/50Hz优点1、孔间温差±1-1.5℃，板面低温度和高温度＜3-5℃2、保证了消解、赶酸的均一性配套器皿消解管（31*100mm）、55ml微波罐（29*160-170mm），其他品牌微波，消解罐内杯，烧杯、坩埚等我司石墨消解器的优点优点1：耐高温耐酸碱及有机溶剂腐蚀，稳定性好；优点2：消解样品速度快，可批量处理样品；优点3：全封闭设计，很大程度防止热量散失的同时，还可有效避免避免酸雾入侵，对设备元件造成损害；优点4：清洁耐腐蚀：采用特别的喷涂工艺，涂层均匀、牢固、长期使用也不会脱落；优点5：采用先进的一体环绕加热方式，样品各部位受热均匀，消解快速；优点6：操作方便，环保节能，节省经济成本；优点7：PID温控系统，性能优良，控温精度高，可达±1℃。优点8：可调节加热速率，实现程序升温并控制加热保持时间，升温速率稳定；仪器的维护1、仪器主机：定期对仪器的电源线及电源线所接电源如插排、墙插等进行检查，如有损坏 老化及时更换。2、清理：将仪器工作面擦拭干净，上面不要有水滴，污物等3、安全：样品处理需要用到各种不同的酸，如HCl、HNO₃、HF等。大部分酸具有挥发性而且对人体不好，因此建议在通风的环境下使用仪器，并做好各种防护措施。4、使用：在说明书指定的工作环境下使用，不用时要拔掉电源，清洁石墨块表面污垢时，要用布轻擦，尽量不使用有机溶剂，不能损坏表面的涂层。5、存储：消解或者加热后，不再用到消解管时应该对其进行清理、并可以到下次实验再次使用，可以节省成本

NanoTemper 推出 MO NT.LabelFree 对照试剂盒，可用于检测配备有 LabelFree 探测器的 MO 系列仪器的性能，或对第一次操作该系统的新用户进行培训。

产品介绍Product Description:bioGenousTMHuman Intestinal Organoid Kit is a chemically defined cell culture medium for establishment and maintenance of human intestinal organoids(hIOs) derived from adult stem cells. Self-renewal of the intestinal epithelium is driven by the proliferation of stem cells and their progenitors located in crypts. Human intestinal organoids display all hallmarks of the intestinal epithelium in terms of architecture, cell type composition, and self-renewal dynamics, therefore hold great promise for unprecedented studies of human intestinal development and disease, human intestinal organoids may also have applications in regenerative biology through ex vivo expansion of the intestinal epithelium.技术参数Product Information:ComponentComponent Cat#VolumeStorage& StabilitybioGenousTMHuman Intestinal Organoid Basal MediumK2002-HI-A100/A500100mL/500 mL4℃，12 monthsbioGenousTMHuman Intestinal Organoid Supplement B(50x)K2002-HI-B100/B5002mL/10 mL-20℃,avoid repeated freeze-thaw cycles, 12 monthsbioGenousTMHuman Intestinal Organoid Supplement C(250x)K2002-HI-C100/C5000.4mL/2 mL-20℃, avoid repeated freeze-thaw cycles, 12 monthsbioGenousTMHuman Intestinal Organoid Supplement D(250x)K2002-HI-D100/D5000.1mL/0.5 mL-20℃, avoid repeated freeze-thaw cycles, 12 monthsPreparation of Human Intestinal Organoid Expansion Medium and Maintenance MediumUse sterile technique to prepare the human intestinal organoid expansion medium and maintenance medium. hIOs grown in Human Intestinal Organoid Expansion Medium overwhelmingly consisted ofLGR5+stem cells, cycling transit amplifying (TA) cells, early enterocytes and a small number of goblet cells. Organoids grown in Human Intestinal Organoid Maintenance Medium contain LGR5+stem cells, TA cells, early and mature enterocytes, goblet cells, M cells and enteroendocrine cells, as well as a low number of Paneth cells and tuft cells. The following examples are for preparing 10 mL of Expansion Medium and Maintenance Medium. If preparing other volumes, adjust accordingly.1.Thaw Human Intestinal Organoid Supplement B(50x), Human Intestinal Organoid Supplement C(250x) and Human Intestinal Organoid Supplement D(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.For Human Intestinal Organoid Expansion Medium. Add 200 μL Human Intestinal Organoid Supplement B(50x), 40 μL Human Intestinal Organoid Supplement C(250x) and 40 μL Human Intestinal Organoid Supplement D(250x) to 9.72 mL Human Intestinal Organoid Basal Medium. Mix thoroughly.3.For Human Intestinal Organoid Maintenance Medium. Add 200 μL Human Intestinal Organoid Supplement B(50x) and 40 μL Human Intestinal Organoid Supplement C(250x) to 9.76 mL Human Intestinal Organoid Basal Medium. Mix thoroughly.NOTE:If not use immediately, store complete medium at 2-8°C for not more than 2 weeks. bioGenousTMHuman Intestinal Organoid Supplement B contains fungicide and antibiotics(50x).Protocol for Establishment of Human Intestinal OrganoidsCAUTIONStudies involving primary human tissue material must follow all relevant institutional and governmental regulations. Informed consent must be obtained from all subjects before the collection of the primary human tissue material.Establishment of Organoids from Primary Tissue1.Collect primary human intestinal 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 or if they also contain fat or muscle tissue. If so, remove non-epithelial components as much as possible using surgical scissors or scalpels and forceps under a dissection microscope. If no fat or muscle tissue are present, continue to the next step immediately.3.Rinse the intestinal tissuewith Epithelial Organoid Basal Medium(B213151) or DPBSuntil the supernatant is clear.4.Before crypt isolation, thaw Matrigel on ice and keep it cold. Add 5 mL of FBS to 45 mL of Epithelial Organoid Basal Medium to prepare 10% (vol/vol) FBS medium.5.Mince the tissue into small fragments of 5 mm3in a cell culture dish using surgical scissors or scalpels.CRITICALThe dissected samples must be small enough to pass through the tip of a 10 mL pipette.6.Place the dissected pieces of sample into a 15 mL conical tube containing 10 mL of cold DPBS.7.Wash the samples by pipetting with a 10 mL pipette at least ten times.CRITICALFor the subsequent steps, coat the inner surface of every 10 mL pipette with 10% (vol/vol) FBS medium before use to avoid adherence of the samples on the pipette wall.8.Stand the tube still until the samples settle at the bottom. Aspirate the supernatant with a 10 mL pipette and add 10 mL of cold DPBS.9.Repeat Steps 7 and 8 3–5 times until the supernatant is free of debris.CRITICALThorough washing of the sample is crucial to avoid bacterial contamination.10.Add 10 mL of cold DPBS supplemented with 2.5 mM EDTA (E219121) to the tube. Place the tube on a rocking shaker and rock it gently at 4 °C for 40 min.11.After treatment with EDTA, stand the tube still until the samples settle to the bottom of the tube, and then aspirate the supernatant with a 10 mL pipette and add 10 mL of cold DPBS.12.Stand the tube still until the samples settle at the bottom. Aspirate the supernatant with a 10 mL pipette.13.Add 10 mL of cold DPBS and pipette up and down at least ten times with a 10 mL pipette. Allowed the tissue fragments to settle down under normal gravity for at least 30s. The crypts will be released into the supernatant by pipetting. Place the supernatant containing the isolated crypts into a new 15 mL tube.14.Spin the crypts at 4°C at 400g for 3 min. Remove the supernatant and place the tube on ice.15.Resuspend the pellet in 1 mL of DPBS and transfer the crypt suspension into a new 1.5 mL tube. Drop 20 μL of the crypt suspension on a petri dish. Count the number of crypts under a stereomicroscope and calculate the total number of crypts.16.Spin the crypts at 4°C at 400g for 3 min. Aspirate and discard the supernatant.17.Aspirate the supernatant and resuspend the pellet in Matrigel. Matrigel should be kept on ice to prevent it from solidifying thus, work quickly. The amount of Matrigel depends on the size of the pellet. Approximately 50-250 crypts should be plated in 25 μL of Matrigel.CRITICALDo not dilute Matrigel too much (Matrigel should be 70% (Matrigel vol/Total vol)) to ensure formation of solid droplets.18.Plate the Matrigel containing organoids on the bottom of 24-well cell culture plates in droplets of ~30 μL each around the center of the well.CRITICALOnce 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.19.Place the culture plate into a humidified incubator at 37 °C and 5% (vol/vol) CO2for15-25 minto let the Matrigel solidify.20.Prepare the required amount of bioGenousTMHuman Intestinal Organoid Expansion Medium.21.Once the Matrigel droplets are solidified (15-25 min), open the plate and carefully add 500 μL of Organoid Complete Medium to each well.CRITICALDo not add the medium directly on top of the Matrigel droplets, as this might disrupt the droplets.22.Place the culture plate in a humidified incubator at 37 °C and 5% (vol/vol) CO2.23.Change the medium every 3 days by carefully aspirating medium from the wells and replacing it with fresh, pre-warmed Organoid Complete Medium.24.Closely monitor the organoid formation. Ideally, human intestinal organoids should be passaged for the first time between 5 and 8 days after initial plating.Splitting and Passaging of Organoids25.Pipette up and down to disrupt the Matrigel, and transfer the organoid suspension into a 1.5 mL conical tube.26.Pipette the organoid suspension up and down to mix thoroughly.Use the bottom of the tube to create pressure, which will aid the removal of Matrigel.27.Centrifuge organoids at 200g for 3 min at room temperature.28.Aspirate the supernatant, and split organoids using either mechanical disruption or Organoid Dissociation Solution (E238001). For mechanical disruption, resuspend the pellet in 1 mL of Organoid Basal Medium. Use a pipette tip to pipette the organoid suspension up and down 30 times. Use the bottom of the tube to create pressure, which will aid organoid disruption. In case of 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 ≥10 times every 1 min to aid in the disruption of the organoids. Monitor digestion closely to keep the incubation time inOrganoid Dissociation Solution to a minimum.CRITICALDo not dissociate in Organoid Dissociation Solution for 3 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.29.After shearing is complete, wash once by topping up with 1 mL ofOrganoid Basal Medium, and centrifuge at 200g for 3 min at room temperature.30.Aspirate the supernatant and resuspend the organoid pellet in 70% (vol/vol) Matrigel, and plate organoids in droplets on the bottom of a culture plate as describedin Steps 12. After plating is complete, transfer the plate into a humidified incubator at 37 °C and 5% (vol/vol) CO2for 15–25 min.31.Pre-warm Human Intestinal Organoid Maintenance Medium at 37 °C.32.After the Matrigel droplets have solidified (15–25 min), carefully pipette pre-warmed medium into the wells.33.Place culture plates in a humidified incubator at 37 °C and 5% (vol/vol) CO2 until the organoids are needed for further experiments.

EPY0000271 奥沙利铂 Oxaliplatin 250 mg EPY0000272 奥沙利铂杂质B Oxaliplatin impurity B 20 mg EPY0000273 奥沙利铂杂质C Oxaliplatin impurity C 15 mg EPY0000274 奥沙利铂杂质D Oxaliplatin impurity D 5 mg EPY0000275 二氯二氨基环己基铂 Dichlorodiaminocyclohexaneplatinum 10 mg EPY0000276 异丙托溴铵杂质A Ipratropium bromide impurity A 5 mg EPY0000277 硫酸粘杆菌素 Colistin sulphate 25 mg EPY0000279 三丁基磷 Tri-n-butyl phosphate 300 µ L EPY0000280 硫酸软骨素钠 Chondroitin sulphate sodium 250 mg EPY0000281 帕罗西汀盐酸盐水合物 Paroxetine hydrochloride hemihydrate 200 mg EPY0000282 噻康唑系统适用性 Tioconazole for system suitability 50 mg EPY0000283 尼麦角林杂质A Nicergoline impurity A 10 mg EPY0000284 丙酸氟替卡松 Fluticasone propionate 100 mg EPY0000288 吡拉西坦 Piracetam 120 mg EPY0000297 美沙拉嗪 Mesalazine 125 mg EPY0000298 辛酸氟奋乃静 Fluphenazine octanoate 10 mg EPY0000299 氟奋乃静亚砜 Fluphenazine sulphoxide 10 mg EPY0000304 天冬氨酸精氨酸 Arginine aspartate 20 mg EPY0000305 天门冬胺酸 Asparagine monohydrate 60 mg EPY0000306 阿奇霉素 Azithromycin 200 mg EPY0000307 阿奇霉素杂质A Azithromycin impurity A 10 mg EPY0000309 布美他尼杂质A Bumetanide impurity A 5 mg EPY0000310 布美他尼杂质B Bumetanide impurity B 5 mg EPY0000311 盐酸塞利洛尔 Celiprolol hydrochloirde 10 mg EPY0000312 塞利洛尔杂质I Celiprolol impurity I 0,02 mg EPY0000313 氯法齐明 Clofazimine 150 mg

SA990620 E10156 钨酐氧化铝，颗粒状 25 g天津欧捷科技有限公司---进口元素分析耗材供应商 天津欧捷科技是一家高科技企业，公司集贸易、科研、服务一体化。公司从精密仪器设备及配件、耗材、试剂、标准对照品、实验室常用耗材的销售，到仪器调试、维护、样品的分析测试。 实验室耗材 元素分析耗材 色谱分析耗材 质谱耗材样品容器 Labco顶空进样瓶 色谱瓶 石英棉 石英燃烧管 进样隔垫 催化剂 标准品 试剂 玻璃碳产品 仪器配件这些耗材可用在Thermo、Elementar、Agilent、Analytikjena、Sercon、Shimadzu、leco、Varian、Perkin Elmer、waters 、Euro Vector等仪器。

SA990620Tungsten oxide / alumina granular 钨酐氧化铝，颗粒状 25 gThermo 33835420Eurovector E10156Hekatech HE33835420Costech 011009 天津欧捷科技有限公司--进口元素分析耗材供应商 保证质量天津欧捷科技是一家高科技企业，公司集贸易、科研、服务一体化。公司从精密仪器设备及配件、耗材、试剂、标准对照品、实验室常用耗材的销售，到仪器调试、维护、样品的分析测试。我们主要经营： 实验室耗材 元素分析耗材 色谱分析耗材 质谱耗材样品容器 Labco顶空进样瓶 色谱瓶 石英棉 石英燃烧管 进样隔垫 催化剂 标准品 试剂 玻璃碳产品 仪器配件这些耗材可用在Thermo、Elementar、Agilent、Analytikjena、Sercon、Shimadzu、leco、Varian、Perkin Elmer、waters 、Euro Vector等仪器。

高效液相色谱法测定土荆皮中土荆皮乙酸的含量 推荐色谱柱 Cosmosil C8-MS 关键词：土荆皮乙酸，辛烷基硅胶键合硅胶，对照品溶液，供试品溶液，高效液相色谱 土荆皮乙酸含量测定，照高效液相色谱法（附录Ⅵ D）测定。 色谱条件与系统适用性试验：以辛烷基硅烷键合硅胶为填充剂；以甲醇-醋酸溶液为流动相；检测波长为260nm。理论板数按土荆皮乙酸峰计算应不低于5000. 土荆皮中土荆皮乙酸含量测定，照高效液相色谱法（附录Ⅵ D），分别精密吸取对照品溶液与供试品溶液，注入液相色谱仪，测定，即得。本品按干燥品计算，含土荆皮乙酸（C23H28O8）不得少于0.25%。（中国药典2010版） 需要详细的药典标准请联系北京绿百草：010-51659766. 登录网站获得更多产品信息:www.greenherbs.com.cn

类器官（Organoids）是指将成体干细胞或多能干细胞在体外三维培养形成的具有一定空间结构的组织类似物。类器官在组织结构、细胞类型、自我更新能力和功能等方面与来源组织高度一致，从而在发育生物学、疾病造模、精准医学、药物研发、基因和细胞疗法、感染和免疫以及再生医学等生物医学的多个领域展现出独特的优势。产品介绍Product Description:bioGenousTMHuman Liver Ductal Organoid Kit is a chemically defined cell culture medium for establishment and maintenance of human liver ductal organoids(hLDs) derived from introhepatic cholangiocyte. Self-renewal of the ductal epithelium is driven by the proliferation of stem cells and their progenitors located in liver. hLDs display all hallmarks of the ductal epithelium in terms of architecture, cell type composition, and self-renewal dynamics, therefore hold great promise for unprecedented studies of human liver development and disease, hLDs may also have applications in regenerative biology through ex vivo expansion of the ductal epithelium.技术参数Product Information:ComponentComponent Cat#VolumeStorage& StabilitybioGenousTMHuman Liver Ductal Organoid Basal Medium(expansion)K2008-HLD –A100/A500100mL/500mL4℃，12 monthsbioGenousTMHuman Liver Ductal Organoid Supplement B(50x)(expansion)K2008-HLD –B100/B5002mL/10mL-20℃,avoid repeated freeze-thaw cycles, 12 monthsbioGenousTMHuman Liver Ductal Organoid Supplement C(250x)(expansion)K2008-HLD–C100/C5000.4mL/2mL-20℃, avoid repeated freeze-thaw cycles, 12 monthsPreparation of Human Liver Ductal Organoid Expansion Medium and Maintenance MediumUse a sterile technique to prepare the human liver ductal organoid expansion medium and maintenance medium. hLDs grown in Human Liver Ductal Organoid Expansion Medium overwhelmingly consisted of cholangiocytes. The following example is for preparing 10 mL Expansion Medium and Maintenance Medium. If preparing other volumes, adjust accordingly.1.Thaw Human Liver Ductal Organoid Supplement B(50x)(Expansion), Human Liver Ductal Organoid Supplement C(250x) (Expansion)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.For Human Liver Ductal Organoid Expansion Medium. Add 200 μL Human Liver Ductal Organoid Supplement B(50x)(Expansion), 40 μL Human Liver Ductal Organoid Supplement C(250x)(Expansion) to Human Liver Ductal Organoid Basal Medium(Expansion). Mix thoroughly.NOTE:If not use immediately, store complete medium at 2-8°C for not more than 2 weeks. bioGenousTMHuman Liver Ductal Organoid Supplement B (Expansion) contains fungicide and antibiotics(50x).Protocol for Establishment of Human Liver Ductal OrganoidsCAUTIONStudies involving primary human tissue material must follow all relevant institutional and governmental regulations. Informed consent must be obtained from all subjects before the collection of the primary human tissue material.Establishment of Organoids from Primary Tissue1.Collect primary human liver 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 or if they also contain fat or muscle tissue. If so, remove non-epithelial components as much as possible using surgical scissors or scalpels and forceps under a dissection microscope. If no fat or muscle tissue are present, continue to the next step immediately.3.Rinse the liver tissuewith Epithelial Organoid Basal Medium(B213151) or DPBSuntil the supernatant is clear.4.Before ducts isolation, thaw Matrigel on ice and keep it cold. Add 5 mL of FBS to 45 mL of Epithelial Organoid Basal Medium to prepare 10% (vol/vol) FBS medium.5.Mince the tissue into small fragments of 5 mm3in a cell culture dish using surgical scissors or scalpels.CRITICALThe dissected samples must be small enough to pass through the tip of a 10 mL pipette.6.Place the dissected pieces of sample into a 15 mL conical tube containing 10 mL of coldEpithelial Organoid Basal Mediumwith 1% FBS.7.Wash the samples by pipetting with a 10 mL pipette at least ten times.CRITICALFor the subsequent steps, coat the inner surface of every 10 mL pipette with 10% (vol/vol) FBS medium before use to avoid adherence of the samples on the pipette wall.8.Stand the tube still until the samples settle at the bottom. Aspirate the supernatant with a 10 mL pipette and add 10 mL of pre-warmed Tissue Digestion Solution (K601008).9.Digest the tissue fractions in 37℃with rotation at the speed of 100 rpm. The digestion time should not exceed 30 mins.CRITICALTo prevent over-digestion, one should examine under the microscope if the duct structure appear during digestion.10.Once the duct structure appears, stop digestion by transfer the digestion solution into 50mL tube and add 40 ml Epithelial Organoid Basal Medium with 1% FBS.11.Stand the tube for 2 min. Transfer the supernatant into a new tube.12.Spin the supernatant at 4°C at 300g for 3 min. Aspirate and discard the supernatant.13.Re-suspend the pellet with 10 ml DMEM with 1%FBS, and spin at 4°C at 300g for 3 min.14.Repeat last step for 2 times.15.Aspirate the supernatant and resuspend the pellet in Matrigel. Matrigel should be kept on ice to prevent it from solidifying thus, work quickly. The amount of Matrigel depends on the size of the pellet. Approximately 20-100 ducts should be plated in 25 μL of Matrigel.CRITICALDo not dilute Matrigel too much (Matrigel should be 70% (Matrigel vol/Total vol)) to ensure formation of solid droplets.16.Plate the Matrigel containing organoids on the bottom of 24-well cell culture plates in droplets of ~30 μL each around the center of the well.CRITICALOnce 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.17.Place the culture plate into a humidified incubator at 37 °C and 5% (vol/vol) CO2 for15-25 minto let the Matrigel solidify.18.Prepare the required amount of bioGenousTMHuman Liver Ductal Organoid Expansion Medium.19.Once the Matrigel droplets are solidified (15-25 min), open the plate and carefully add 500 μL of Organoid Complete Medium to each well.CRITICALDo not add the medium directly on top of the Matrigel droplets, as this might disrupt the droplets.20.Place the culture plate in a humidified incubator at 37 °C and 5% (vol/vol) CO2.21.Change the medium every 3 days by carefully aspirating medium from the wells and replacing it with fresh, pre-warmed Organoid Complete Medium.22.Closely monitor the organoid formation. Ideally, human liver ductal organoids should be passaged for the first time between 5 and 8 days after initial plating.Splitting and Passaging of Organoids23.Pipette up and down to disrupt the Matrigel, and transfer the organoid suspension into a 1.5 mL conical tube.24.Pipette the organoid suspension up and down to mix thoroughly.Use the bottom of the tube to create pressure, which will aid the removal of Matrigel.25.Centrifuge organoids at 200g for 3 min at room temperature.26.Aspirate the supernatant, and split organoids using either mechanical disruption or Organoid Dissociation Solution (E238001). For mechanical disruption, resuspend the pellet in 1 mL of Organoid Basal Medium. Use a pipette tip to pipette the organoid suspension up and down 30 times. Use the bottom of the tube to create pressure, which will aid organoid disruption. In case of 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 ≥10 times every 1 min to aid in the disruption of the organoids. Monitor digestion closely to keep the incubation time inOrganoid Dissociation Solution to a minimum.CRITICALDo not dissociate in Organoid Dissociation Solution for 3 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.27.After shearing is complete, wash once by topping up with 1 mL ofOrganoid Basal Medium, and centrifuge at 200g for 3 min at room temperature.28.Aspirate the supernatant and resuspend the organoid pellet in 70% (vol/vol) Matrigel, and plate organoids in droplets on the bottom of a culture plate as describedin Steps 12. After plating is complete, transfer the plate into ahumidified incubator at 37 °C and 5% (vol/vol) CO2for 15–25 min.29.Pre-warm Human Liver Ductal Organoid Maintenance Medium at 37 °C.30.After the Matrigel droplets have solidified (15–25 min), carefully pipette pre-warmed medium into the wells.31.Place culture plates in a humidified incubator at 37 °C and 5% (vol/vol) CO2until the organoids are needed for further experiments.

食品烘干房除湿机 新闻资讯报道：在食品加工过程中，烘干或干燥工艺是其中最难以掌握的一道生产工艺,与食品的质量，企业的经济效益都是息息相关的！现如今，对于干燥食品的需求是越来越多，不仅重视其食品的口感，也越来越重视食品的营养成分。烘干或干燥技术的好坏对食品口感及其营养风味都是有很大影响的；在以往，大多依靠自然通风和日晒可以达到食品干燥的目的，但受自然条件约束，且食品卫生难以保证。还有的则采用机械通风、加热烘干能使生产条件有所改善，但对动物类食品加工过程中，易发生油脂氧化现象，表面变黄，并带有辣味，产品质量下降。而且在食品的烘干过程中，食品中的水分会不断的蒸发到烘干房中,水蒸气会不断的增多，如果不及时的排出，不仅会影响烘干的效率，还会影响食品的口感和品质！在以往，很多食品加工厂或企业在烘干房中安装排风机来将水蒸气排出去，但在排出水蒸气的同时，热量也随之排出， 大量的热能白白浪费掉， 大大增加了烘干房的运行产成本。为此，现在已经有不少的食品加工厂或企业开始使用正岛ZD-8240G食品烘干房除湿机及ZD系列耐高温除湿机来对烘干房进行除湿，能够快速的，及时的去除烘干房内的水蒸气；大大提高了食品烘干的效率，以及其品质和安全！ 比如：某烘干房内在烘干过程中由于湿度大，采用了通风排湿的方法，烘干的时间需要24小时；而正岛ZD-8240G食品烘干房除湿机及ZD系列耐高温除湿机后，则可以在不排出热量的情况下快速降低烘干房内的湿度；那么，现在只需要16小时或12小时即可达到原来24小时的烘干效果，大大降低了烘干房的运行成本。现已在全国各地的工厂企业烘干房内推广使用，其效果也得到了所有用户的认可。一般冷冻式除湿机的工作环境温度为5-38℃，超过38℃除湿机将实施自动保护而停机。但在物料干燥室，烘干房内，其室内温度一般超过40℃，所以一般的冷冻式除湿机无法在此环境下工作。现在一般企业的物料干燥方法是将干燥室，烘干房内湿热空气通过风机强行外排。这样，室内的热量也随之排出室外。针对干燥室、烘干房节能除湿干燥的需求，正岛电器专门开发出正岛ZD-8240G食品烘干房除湿机及ZD系列耐高温除湿机(适用于室内温度高于38℃低于55℃的环境下除湿)； 可广泛应用于制药、化工、食品、轻工、重工等行业物料及产品的加热固化、干燥脱水。如：木材、干果类、食用菌类、农副产品、纸制品、原料药、生药、中药饮片、粉剂、颗粒、冲剂、颜料、染料、脱水蔬菜、瓜果干、香肠、塑料树脂、电器原件、烘漆等。欢迎您来电咨询食品烘干房除湿机的详细信息！耐高温除湿机的种类有很多,不同品牌的耐高温除湿机价格及应用范围也会有细微的差别,而我们将会为您提供优质的产品和全方位的售后服务。备注：该系列产品可与环境试验设备以及环境监测仪器等温湿度相关仪器设备配套使用，也可作为其中的一个核心配件！正岛ZD-8240G食品烘干房除湿机及ZD系列耐高温除湿机技术参数： 注：工作环境温度要求5～55℃； 最高可进风温度≤55℃产品型号除湿量(L/D)功率(W)风量（m3/h ）电源(V/HZ)尺寸(mm)净重(kg)ZD-8168G16828002100380V~50Hz605X410X1650126ZD-8240G24049003000380V~50Hz770X470X1650160ZD-8360G36070004500380V~50Hz1240X460X1700255ZD-8480G48099006000380V~50Hz1240X460X1750300压缩机 耐高温型涡旋式压缩机 非标定制 管道式&吊顶式 耐高温除湿机选型：根据实际的烘干房的总体湿负荷来选配最适合的型号，具体的就是根据其面积，层高，以及烘干水分的蒸发量，初始湿度值目标湿度值，还有室内的密闭效果，散湿源，新风补给等综合因素来计算出制冷量，单位时间的除湿量等其它关键数据后才能正确的选出需要的型号。本站新闻记者核心提示：正岛ZD-8240G食品烘干房除湿机及ZD系列耐高温除湿机适用于菊花，大枣，金银花,海带、紫菜、鱼干、虾米、鱿鱼、鱼片，海参，鲍鱼等海产品烘干， 也适用于笋干、菌类、大蒜、花卉、干果、蔬菜、香菇、地瓜、玉米、豌豆 ，豆角、椰子、槟榔、木耳等农副产品的烘干， 以及金银花、菊花、大黄、丹参，人参等中药材烘干房中进行合理的除湿！ 烘干技术是提高烘干或干燥食品质量的重要途径之一。在各种食品的烘干过程中,含水率控制主要依据烘干房内温度和湿度的变化；那么，对加热和排湿这两个方法要进行严格的控制，不但确保了烘干工艺的持续进行,提高食品的烘干或干燥品质,而且还可以提高食品烘干房的烘干效率和产量；与此同时，还能大大降低烘干的生产成本！因此，在食品烘干房中配上一台正岛ZD-8240G食品烘干房除湿机及ZD系列耐高温除湿机来进行合理的除湿是非常有要的！以上关于食品烘干房除湿机的全部新闻资讯是正岛电器为大家提供的！

类器官（Organoids）是指将成体干细胞或多能干细胞在体外三维培养形成的具有一定空间结构的组织类似物。类器官在组织结构、细胞类型、自我更新能力和功能等方面与来源组织高度一致，从而在发育生物学、疾病造模、精准医学、药物研发、基因和细胞疗法、感染和免疫以及再生医学等生物医学的多个领域展现出独特的优势。产品介绍Product Description:bioGenousTMHuman Liver Ductal Organoid Kit is a chemically defined cell culture medium for establishment and maintenance of human liver ductal organoids(hLDs) derived from adult stem cells. Self-renewal of the liver ductal epithelium is driven by the proliferation of stem cells and their progenitors located in liver. hLDs display all hallmarks of the liver ductal epithelium in terms of architecture, cell type composition, and self-renewal dynamics, therefore hold great promise for unprecedented studies of Human liver development and disease, hLDs could differentiate into hepatocyte like cell under the induction of differentiation medium.技术参数Product Information:ComponentComponent Cat#VolumeStorage& StabilitybioGenousTMHuman Liver Ductal Organoid Basal Medium（Differentiation）K2008-HLH –A100/A500100mL/500mL4℃，12 monthsbioGenousTMHuman Liver Ductal Organoid Supplement B(50x)（Differentiation）K2008-HLH –B100/B5002mL/10mL-20℃,avoid repeated freeze-thaw cycles, 12 monthsbioGenousTMHuman Liver Ductal Organoid Supplement C(250x)（Differentiation）K2008-HLH –C100/C5000.4mL/2mL-20℃, avoid repeated freeze-thaw cycles, 12 monthsbioGenousTMHuman Liver Ductal Organoid Supplement D(250x)（Differentiation）K2008-HLH –D100/D5000.4mL/2mL-20℃, avoid repeated freeze-thaw cycles, 12 monthsPreparation of Human Liver Ductal Organoid Differentiation MediumUse sterile technique to prepare the human liver ductal organoid differentiation medium. hLDs grown in Human Liver Ductal Organoid Expansion Medium overwhelmingly consisted of cholangiocytes. After changing the Expansion Medium to differentiation medium, the hLDs could differentiate into hepatocyte like cells, which display the markers of hepatocytes, includingALBUMIN,TTRandCYP3A4. The following examples are for preparing 10 mL of Differentiation I Medium and Differentiation II Medium. If preparing other volumes, adjust accordingly.1.Thaw Human Liver Ductal Organoid Supplement B(50x) (Differentiation), Human Liver Ductal Organoid Supplement C(250x) (Differentiation) and Human Liver Ductal Organoid Supplement D(250x) (Differentiation) on ice.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.For Human Liver Ductal Organoid Differentiation Medium I. Add 40 μL Human Liver Ductal Organoid Supplement D(250x) (Differentiation) to 10 mL Human Liver Ductal Organoid Medium(Expansion) (K2008-HLD). Mix thoroughly.3.For Human Liver Ductal Organoid Differentiation Medium II. Add 200 μL Human Liver Ductal Organoid Supplement B(50x) (Differentiation) and 40 μL Human Liver Ductal Organoid Supplement C(250x)（Differentiation）to 10 mL Human Liver Ductal Organoid Basal Medium (Differentiation). Mix thoroughly.NOTE:If not use immediately, store complete medium at 2-8°C for not more than 2 weeks. bioGenousTMHuman Liver Ductal Organoid Supplement B (Differentiation) contains fungicide and antibiotics(50x).

枯草杆菌黑色变种芽孢指示菌片-----环氧乙烷和干热灭菌效果的监测 本枯草杆菌黑色变种芽孢生物指示剂菌片是由枯草杆菌黑色变种（ATCC 9372）芽孢和特种滤纸片组成。菌片回收菌量为5.0× 105 cfu/片～5.0× 106 cfu/片。 生物指示剂菌片的抗力符合国际标准和国家标准的规定： 对环氧乙烷的抗力标准，在环氧乙烷剂量为600 mg/L± 30 mg/L，作用温度54℃，相对湿度60％± 10％条件下，存活时间&ge 7.8 min，死亡时间&le 58 min，D10值5.8 min。 对干热的抗力标准，在160℃干热条件下，存活时间&ge 3.9 min，杀灭时间&le 19 min，D10值1.3 min～1.9 min。 【型 号】指示菌片 【使用范围】该生物指示剂菌片可用于对环氧乙烷和干热灭菌效果的监测。 【使用方法】 1 用于环氧乙烷和干热灭菌效果监测时，将生物指示剂菌片置于小纸袋内，按《医院消毒供应中心：清洗消毒及灭菌效果监测标准（WS 310.3-2009）》的要求放入物品包内，置于适当位置，进行灭菌处理。检测同时设生物指示剂菌片阳性对照，阳性对照生物指示剂菌片放室温下，不进行灭菌处理。 2 灭菌完毕，在无菌操作下取出小纸袋中的生物指示剂菌片，投入无菌普通营养肉汤管内，同时将未经灭菌处理的生物指示剂菌片投入另一支无菌普通营养肉汤管内，作为阳性对照，置37℃恒温培养箱内连续培养7 d，逐日观察结果。 【结果判定】培养后普通营养肉汤液面有菌膜，普通营养肉汤内有絮状沉淀，摇动时见有混浊，即表示有菌生长，判定为灭菌不合格；培养后普通营养肉汤仍澄清透明且无沉淀即表示无菌生长，同时阳性对照生物指示剂菌片生长正常，判定为灭菌合格。 【注意事项】 1 本生物指示剂菌片的检验须按《医院消毒供应中心：清洗消毒及灭菌效果监测标准（WS 310.3-2009）》的要求进行。 2 本生物指示剂菌片应保存于4℃冰箱内。 【有 效期】 12个月。 【包装规格】 50片/包。 附录：普通营养肉汤培养基的制备 【营养肉汤培养基配方】牛肉膏5 g，蛋白胨10 g，氯化钠5 g，蒸馏水。 【制备方法】 1 牛肉膏5 g，蛋白胨10g，氯化钠5 g，溶于900 ml蒸馏水中。 2 调节pH 值为7.2～7.4, 补充蒸馏水至1000 ml。 3 分装后，置121℃压力蒸汽灭菌20 min或115℃压力蒸汽灭菌30 min。放入4℃冰箱内保存，备用。

配件编号：A0941-040产品名称：Tubing 1/16英寸 OD 10 ID 9L SS产品规格：A0941-040仪器厂商：ThermoFisher/热电价格：面议库存：是配件编号：A037318产品名称：升降杆传送皮带产品规格：A037318仪器厂商：ThermoFisher/赛默.飞世尔价格：面议应用于直读光谱仪 ARL 9800配件编号：A0941-060产品名称：Tubing 1/16英寸 OD 10 ID 4L SS产品规格：A0941-060仪器厂商：ThermoFisher/热电价格：面议库存：是

HUP系列超声波细胞破碎仪配件如下：1、隔音箱。2、支架。3、降温冷却细胞器。4、升降台。5、变幅杆工具头。变幅杆工具头规格如下：1/8〃,1/4〃,3/8〃,1/2〃

石墨赶酸器、石墨赶酸电热板一、产品介绍石墨赶酸器又称赶酸板、样品处理器、赶酸仪、消解器。适用于食品、疾控、农科院、医药、农业、林业、环保、化工、生化等行业以及高等院校、科研部门对微波消解、高压消解的后期赶酸,是原子吸收、原子荧光、ICP- AES、AA、ICP- MS等分析仪器的理想配套产品。石墨赶酸器参数型 号ZH控温范围室温-260℃控温精度±0.1℃，最高温度差3-5℃加热材质优质石墨+特氟龙防腐涂层样品孔数20、25、30、40、42、48孔等（可根据客户要求加工定制）控显方式PID控温数显电 源220v/50Hz优点1、孔间温差±1-1.5℃，板面低温度和高温度＜3-5℃2、保证了消解、赶酸的均一性配套器皿消解管（31*100mm）、55ml微波罐（29*160-170mm），其他品牌微波，消解罐内杯，烧杯、坩埚等我司石墨消解器的优点优点1：耐高温耐酸碱及有机溶剂腐蚀，稳定性好；优点2：消解样品速度快，可批量处理样品；优点3：全封闭设计，很大程度防止热量散失的同时，还可有效避免避免酸雾入侵，对设备元件造成损害；优点4：清洁耐腐蚀：采用特别的喷涂工艺，涂层均匀、牢固、长期使用也不会脱落；优点5：采用先进的一体环绕加热方式，样品各部位受热均匀，消解快速； 优点6：操作方便，环保节能，节省经济成本； 优点7：PID温控系统，性能优良，控温精度高，可达±1℃。优点8：可调节加热速率，实现程序升温并控制加热保持时间，升温速率稳定；仪器的维护1、仪器主机：定期对仪器的电源线及电源线所接电源如插排、墙插等进行检查，如有损坏 老化及时更换。2、清理：将仪器工作面擦拭干净，上面不要有水滴，污物等3、安全：样品处理需要用到各种不同的酸，如盐酸、HNO₃ 、HF等。大部分酸具有挥发性而且对人体不好，因此建议在通风的环境下使用仪器，并做好各种防护措施。4、使用：在说明书指定的工作环境下使用，不用时要拔掉电源，清洁石墨块表面污垢时，要用布轻擦，尽量不使用有机溶剂，不能损坏表面的涂层。5、存储：消解或者加热后，不再用到消解管时应该对其进行清理、并可以到下次实验再次使用，可以节省成本。安全使用及注意事项1、 使用含HClO4的消解剂时，控制好HClO4量和消解温度等条件，安全才有保障，否则有燃烧、爆炸的危险。2、 在操作仪器时出现安全问题，立刻关闭仪器，禁止继续操作。3、 由于加热H₂ SO₄ 、盐酸等消解液及样品，消化管温度比较高，小心灼伤。4、 在操作仪器的时候，要穿着防护设备和佩带护眼罩。5、 仪器出现故障时，及时与厂家联系。

杭州卓祥毛细管粘度计型号齐全,包括乌氏粘度计、品氏（平氏）粘度计等，精密度高，易填充，性能稳定，与国际技术同步，可根据用户所规定的规格进行生产常见乌氏粘度计的毛细管直径、K值和测量范围对照表：尺寸编号毛细管内径(mm)运动粘度范围（mm2/s）K值00.240.3-10.0010C0.360.6-30.0030B0.461~50.0050A0.501.5-710.582~100.011C0.78(0.77)6-300.031B0.8810-500.0521.0320-1000.12C1.3660-3000.32B1.55100-5000.52A1.71150-75031.83200-10001.03C2.43600-30003.03B2.751000-50005.043.272000-10000104C4.326000-30000304B5.2010000-500005056.2520000-100000100

【产品名称】：MID芽孢杆菌鉴定系统（MID-66）【英文名称】：MID Bacillus【产品说明】：MID Bacillus是用于鉴定从食品和食品原料中分离出来的嗜常温芽孢杆菌 (Mesophilic Bacillus spp)的鉴定系统。【储存方式】：未开封的试验条以及芽孢杆菌悬浮肉汤储存于2-8℃条件，可保藏至使用有效期。【产品原理】： MID Bacillus由两条生化反应条组成（标明 BAC 1 和 BAC 2），每条有12个反应小管，小管中装有干燥底物，用于碳水化合物发酵反应和其他反应试验。第二条鉴定条最后一个反应管作为糖发酵空白标准对照。该鉴定条所选择的底物是经过电脑分析选择适用于鉴定和鉴别此菌群的底物进行设计的。 在30℃条件下培养，分别在24、48小时记录结果，并在48小时添加配套试剂（Indole, Nitrate 和 VP tests），记录最后的结果。 将记录结果输入MID鉴定系统软件 (MID-60) 进行分析产品特点： 专为芽孢杆菌属设定的鉴定系统。 鉴定试剂依据传统方法，并已在大量科学论文中得到充分验证 24个生化反应的测试条，操作简单，易于使用 48h获得鉴定结果 使用Mircogen公司的鉴定系统软件分析结果鉴定试剂：铝箔袋独立包装的20套鉴定条（MID66c）（BAC1 和 BAC2）， 20瓶MID66b芽孢杆菌悬浮培养基，反应条培养槽，结果记录报告单，使用说明书。其它必备品：MID鉴定系统软件 (MID-60) 1.1.16.19版本或以上， 矿物油（或无菌液体石蜡油）， VP I 和 VP II 试剂， Nitrate A&B试剂， Kovac试剂， 血琼脂/营养琼脂平板， 革兰氏染液， 触酶反应试剂。鉴定流程:Bacillus ID系统是用于鉴定从食物和食物原料中分离出来的嗜常温芽孢杆菌 (Mesophilic Bacillus spp)。注：了解产品更多资料信息请查阅《MID-66芽孢杆菌鉴定使用说明书（MID Bacillus-ID）》！！！

赶酸器GS赶酸器:又称赶酸电热板、赶酸板、样品处理器、赶酸仪、消解器。适用于食品、疾控、农科院、医药、农业、林业、环保、化工、生化等行业以及高等院校、科研部门对微波消解、高压消解的后期赶酸,是原子吸收、原子荧光、ICP- AES、AA、ICP- MS等分析仪器的理想配套产品。技术参数型号GS型孔数、孔径要求可根据客户样品量加工成12 、16、20、24、36、42、54、63、72等位数及特殊孔径×深度的电热板加热方式环绕式电加热 PID数显温控范围室温-200℃控温精度±1℃加热板块表面防腐进口Teflon涂层加热板材质铝合金额定电压220V连续工作时间＞48h配套产品配套美国CEM、配套迈尔斯通、配套利曼、配套上海新仪、配套北分瑞利、配套安东帕、配套上海屹尧等厂家的内罐，配套消解罐内杯、烧杯、试管、坩埚、消解罐内杯、PFA溶样罐等

订货信息：清洗和维护用消耗品　说明部件号一年维护工具包（用于扩散泵系统）包括氦气通用大捕集阱（1/8英寸），砂纸（5/包），不起毛布（15/包）棉签（100/包），SantoVacUltra，18.5mL（2瓶），前级泵油（1升），灯丝组件，八氟萘(OFN)5183-2096尼龙手套，不起毛，大号，1副8650-0030尼龙手套，不起毛，小号，1副8650-0029不起毛工业擦布，100%棉，9x9英寸，300/包9310-4828离子源清洗工具包包括不起毛布（15/包）、砂纸（5/包）、棉签（100/包）、不起毛尼龙手套、研磨用氧化铝粉5181-8863不起毛的布05980-60051棉签，100/包5080-5400砂纸，氧化铝绿色擦拭纸，600目，5/包5061-5896氧化铝粉，研磨，1kg8660-0791检验合格的PFTBA样品，10g8500-0656PFTBA和PFDTD测试样品的可更换玻璃球G3170-80002PFTBA和PFDTD测试样品的可更换玻璃样品瓶05980-20018活性氧化铝，用于Edwards前级泵捕集阱的吸附剂，不用于LC/MS，每罐1lb8500-1233MSD工具包，5975/5973包括离子源支撑工具、无纺布、棉签、无纺尼龙手套、砂纸、扳手和螺丝刀工具G1099-60566MSD工具包，5972/5971包括小清洁杆、大清洁杆、离子源支撑工具、棉签（100/包）、不起毛尼龙手套、砂纸、扳手和螺丝刀工具05971-60561MS接口备件　MS接口柱螺帽，内螺纹05988-20066长密封垫圈或双孔长密封垫圈用柱螺帽05921-21170通用柱螺帽，2/包5181-8830MS 接口色谱柱安装工具，用于5973和5975G1099-200305975T 的色谱柱安装工具G3880-20030工具　螺丝刀，3英寸PozidrivshaftNo.2pt，适合2-4号螺丝8710-0899螺丝刀，4英寸PozidrivshaftNo.2pt，适合5-10号螺丝8710-0900开口扳手，1/4和5/16英寸8710-0510MS接口色谱柱安装工具G1099-20030六角螺母改锥，5.5mm8710-1220螺丝刀，TORXT208710-1615螺丝刀，TORXT158710-1622螺丝刀，TorxT105182-3466密封垫圈　0.4mmVespel/石墨密封垫圈，用于200/250&mu m柱，10/包5062-35080.5mmVespel/石墨密封垫圈，用于320&mu m柱，10/包5062-3506250&mu mVespel/石墨密封垫圈，10/包5181-3323SilTite金属密封圈，用于1/16英寸外径的管线，10/包包含2个柱螺帽5184-3571SilTite金属密封垫圈，1/16英寸x0.4mm内径，10/包包括2个柱螺帽5184-3569SilTite金属密封垫圈，1/16英寸x0.5mm内径，10/包包括2个柱螺帽5184-3570密封圈预成型工具G2855-60200微流控多管系统或两通接头塞G2855-60201

日本SANYO三洋公司HUBY-340棉签，净化棉签，无尘棉签，洁净棉签，净化棉棒 HUBY 棉签由世界著名棉签生产厂商&mdash 日本SANYO公司生产，所有型号棉签均选用优质长丝棉，专业用于各行业精密产品的擦拭、清洁。可在生产过程的特殊环境中（擦拭布无法擦拭）消除污染物和保持清洁。擦拭后化学残留物含量低。可燃，易处理，对环境无害环保。大部分的清洁棉签是导电级的，可保持操作者和工具接地。适用范围：激光及相关工业，半导体及相关产业，光学，电子显微镜，磁读写头的清洗，视频头，磁头的清洗，精密器件等。　 具有如下优点. 　　1、吸附力强，发尘量小，低离子残留 　　2、浸泡溶济后，棉头不易疏松变形 　　3、防静电无硅封装 　　4、环保材质，易于回收 　　5、有多种头型可供选择，以方便擦拭不同类型产品 　　6、独特的防伪标记 HUBY-340 BB-001 净化棉签 3寸 纸杆 双棉头 25支/包 HUBY-340 BB-002 净化棉签3寸 纸杆 双棉头 25支/包 HUBY-340 BB-003 净化棉签 3寸 纸杆 双尖头 25支/包 HUBY-340 BB-012 净化棉签 3寸，纸杆 双棉头 25支/包 HUBY-340 BB-013 净化棉签 3寸，纸杆 双尖头 25支/包 HUBY-340 FS-010 净化棉签 3寸，胶杆 平头25支/包 防静电杆/黑色 HUBY-340 CA-002 净化棉签 3寸，纸杆 双棉头 25支/包 HUBY-340 CA-003 净化棉签 3寸，纸杆 双尖头 25支/包 HUBY-340 CA-005 净化棉签 6寸，纸杆 平单头 100支/包 HUBY-340 CA-006 净化棉签 6寸，木杆 单头 100支/包 HUBY-340 CA-007 净化棉签 6寸，纸杆 双头 100支/包 HUBY-340 CA-008 净化棉签 6寸 纸杆 双尖头 100支/包 HUBY-340 CA-010 净化棉签 6寸 纸杆 单平头 50支/包

糖苷分离技术(GST：Glycan Separation Technology)糖蛋白分析涉及确认复杂的N-和O-端结构，它们通常由相似的和重复的糖片段组成。使用配有荧光检测的亲水作用色谱(HILIC：Hydrophilic-Interaction Chromatography)是受到广泛认可的可靠技术，能够在糖苷被荧光标记衍生化后对它们进行有效的分离和定量。ACQUITY UPLC BEHGlycan色谱柱，专门设计并经过QC测试，为一系列糖苷结构提供在更短时间内进行卓越的UPLC组份分离的能力。再配合ACQUITY UPLC系统，就能帮助用户更快的得到正确的答案。沃特世ACQUITY UPLC BEH Glycan色谱柱，设计用于HILIC模式分离2-氨基苯甲酰胺(2-AB)标记糖苷。该色谱柱的化学性质与我们所推荐的UPLC仪器条件，能够使用一个二元梯度同时分离中性糖苷和带电糖苷。2-AB标记寡糖的保留性取决于该分子的亲水性。该色谱柱的高分辨能力部分来自其小粒径、1.7 μm的多孔填料。色谱柱的化学稳定性和机械稳定性则受益于沃特世的亚乙基桥杂化颗粒技术(BEH)组成和配体键合技术，这有助于确保批次间稳定一致的性能。1、与现有的基于HPLC的方法相比，在更短的时间内实现组份分离度的提高2、配合ACQUITY UPLC系统与荧光检测器时效果最佳3、基于沃特世BEH颗粒和键合技术，可实现对标记糖苷的稳定、可重现的分离4、用相关标记糖苷标准品进行质控测试，以确保稳定的批次间的重现性ACQUITY UPLC BEH Glycan色谱柱分离2-AB标记人IgG糖苷ACQUITY UPLC BEH Glycan色谱柱分离2-AB标记葡聚糖序列ACQUITY UPLC BEH Glycan柱产品描述 柱规格 粒径 部件号ACQUITY UPLC BEH Glycan 2.1 x 50 mm 1.7 μm 186004740ACQUITY UPLC BEH Glycan 2.1 x 100 mm 1.7 μm 186004741ACQUITY UPLC BEH Glycan 2.1 x 150 mm 1.7 μm 186004742ACQUITY UPLC BEH Glycan VanGuard 预柱 — 1.7 μm 186004739ACQUITY UPLC BEH Glycan方法验证包* 2.1 x 100 mm 1.7 μm 186004907*三根柱来自不同的填料批次注意：ACQUITY UPLC BEH Glycan, 1.7μm柱，设计用于ACQUITY UPLC系统。只有具备低系统死体积和低检测器谱带扩散的ACQUITY UPLC系统，才能实现ACQUITY UPLC BEH Glycan柱所装填的1.7μm颗粒的色谱优势。

小号洗耳球，30ml（吹气球、皮老虎） 【名 称】：洗耳球（吹气球、皮老虎） 【规 格】： 小号，30ml，总长约90mm，直径约45mm，重量约21.6克 中号，60ml，总长约100mm，直径约50mm，重量约29.8克 大号，90ml，总长约110mm，直径约60mm，重量约38.3克 每只有单独塑料袋包装。50只一大袋，每箱6袋，共300只。

小号洗耳球，30ml（吹气球、皮老虎） 【名 称】：洗耳球（吹气球、皮老虎） 【规 格】： 小号，30ml，总长约90mm，直径约45mm，重量约21.6克 中号，60ml，总长约100mm，直径约50mm，重量约29.8克 大号，90ml，总长约110mm，直径约60mm，重量约38.3克 每只有单独塑料袋包装。50只一大袋，每箱6袋，共300只。

小号洗耳球，30ml（吹气球、皮老虎） 【名 称】：洗耳球（吹气球、皮老虎） 【规 格】： 小号，30ml，总长约90mm，直径约45mm，重量约21.6克 中号，60ml，总长约100mm，直径约50mm，重量约29.8克 大号，90ml，总长约110mm，直径约60mm，重量约38.3克 每只有单独塑料袋包装。50只一大袋，每箱6袋，共300只。

赶酸器GS赶酸器:又称赶酸电热板、赶酸板、样品处理器、赶酸仪、消解器。适用于食品、疾控、农科院、医药、农业、林业、环保、化工、生化等行业以及高等院校、科研部门对微波消解、高压消解的后期赶酸,是原子吸收、原子荧光、ICP- AES、AA、ICP- MS等分析仪器的理想配套产品。技术参数型号GS型孔数、孔径要求可根据客户样品量加工成12 、16、20、24、36、42、54、63、72等位数及特殊孔径×深度的电热板加热方式环绕式电加热 PID数显温控范围室温-200℃控温精度±1℃加热板块表面防腐进口Teflon涂层加热板材质铝合金额定电压220V连续工作时间＞48h配套产品美国CEM、迈尔斯通、利曼、上海新仪、北分瑞利、安东帕、上海屹尧等厂家的内罐，消解罐内杯、烧杯、试管、坩埚、消解罐内杯、PFA溶样罐等产品特点：1、进口优质PFA 涂层, 一抹即净、永不生锈,特氟隆防腐铸铝加热板升温速度快2、工作温度：室温至260℃，可连续工作48h,5-30分钟可升到200℃（因孔深而异）3、一次性处理样品量大，用时短，与只是靠平面供热辐射立面的一般孔式消解仪相比，能够提高50%的工作效率4、环绕式加热，孔间温差小，加热均匀，使用方便，寿命长。5、板面与控制盒可以做成分体式，裸露部分都采用PFA管子包裹，这样在实验过程中的酸雾就不会腐蚀控制盒里的元器件，从而增加了使用寿命，多个样品同时处理无交叉污染6、消解均匀：器皿底部及360°包裹式加热，使得样品加热无盲点，稳定性好，均匀性很好8、仪器周围可增置外壳，美观且保温用途：专为实验室设计的，是样品加热消解、蒸酸、煮沸、赶酸的好帮手，也是原子吸收，原子荧光等分析仪器的理想配套产品。可以检测食品、药品、乳制品等等中铅、镉、铬、汞、砷、锌、硒、锰等重金属元素，以及微量元素；测定土壤中重金属和微量元素的消解等。