BLM系列磁珠规格书

免疫磁珠链霉亲和素磁珠（免疫捕捉、纯化）100~500nm免疫磁珠 |链霉亲和素磁珠(免疫捕捉、纯化) 100~500nm关键词：免疫磁珠、链霉亲和素磁珠(免疫捕捉、纯化) 100~500nm免疫磁珠、链霉亲和素磁珠 (免疫捕捉、纯化) 1umSera-Mag™ 链霉亲和素磁珠和 SpeedBeads链霉亲和素磁珠可用于捕获生物素化靶分子，进行快速和可靠的蛋白质组学分析。

Sera-Mag™ and Sera-mag SpeedBeads 链霉亲和素磁珠，对于生物素化靶分子显示出较高亲和力和灵敏度，具有快速反应动力学，从而可以提高基因组学和蛋白质组学应用的通量和精密度。

性质：具有较低（2500 至3500 pmol/mg）、中等（3500 至4500 pmol/mg）或较高（4500 至 5500 pmol/mg）生物素结合载量，优化测定开发较低解离常数确保紧密的配基结合较低非特异性结合可实现更高的精密度和准确度结合了大比表面积、高灵敏度、物理性能稳定性和快速反应动力学的特点均匀的链霉亲和素涂层可获得可靠结果粒径均一，1um 的粒径可提供较大比表面积和出色的批次间重现性。

Sera-Mag™ SpeedBeads 和Sera-Mag™ 链霉亲和素磁珠，不仅有快速反应动力学，而且有较低的非特异性结合，可提高免疫测定和分子生物学应用（如用于基因组学和蛋白质组学的样品制备和测定开发）中的通量和精密度。

【成分】亲和素包覆的磁性氧化铁纳米球，含1%BSA的硼酸缓冲液【性状】黑褐色悬液，长时间静置可分层【特点与用途】链霉亲和素磁珠由超顺磁性微球与高纯度链霉亲和素共价结合而成。

链霉亲和素-生物素（SA-Biotin）系统具有极高的结合亲和力（Kd=10^-15），在生物领域具有广泛的应用。

本产品采用超顺磁性微球，粒径均一、形貌规整，有利于方便、快捷地捕获目标分子以及实现磁性分离。

【基本使用方法】在室温条件下，将生物素化抗体与链酶亲和素磁性微球混合，反应时间30~40min，制备成磁性微球探针；将制备好的磁性微球探针与带检测分离的样品混合，再用磁力架进行磁性分离清洗。

提供村田磁珠规格书村田电容规格书村田电感规专业销售日本村田MURATA品牌电子元器件.村田电容,村田贴片电容,村田陶瓷电容,村田安规电容,村田可调电容,村田电感,村田贴片电感,村田绕线电感,村田叠层电感,村田高频电感,村田功率电感,村田屏蔽电感,村田薄膜电感,村田磁珠,村田贴片磁珠,村田EMI磁珠,村田EMI滤波器,村田声表滤波器,村田蓝牙滤波器,村田陶瓷振荡子.村田三端子滤波器,村田热敏电阻,村田NTC热敏电阻,村田贴片热敏电阻.村田射频头,村田射频测试线,村田RF同轴连接器,村田传感器等等.并提供相应产品规格书.选型指南.村田代理现货供应日本村田MURATA 电子元器件贴片陶瓷电容常用料如下：GRM155R61C104KA88D、GRM155R61A105KE15D、GRM155R60J225ME15D 、GRM185R61C105KE44DGRM188R61C105KA93D、GRM188R60J225KE19D 、GRM188R61A225KE34D 、GRM188R60J475KE19DGRM188R71A225KE15D、GRM188R60J106ME47D 、GRM21BR71C105KA01L、GRM219R60J106KE19DGRM21BR60J106KE19L、GRM219R60J226ME47D 、GRM21BR60J226ME39L、GRM31CR61E106KA12LGRM32ER61C476KE15L、GRM32ER60J107ME20L、GNM214R61A105ME17D、GNM1M2R61C105ME18D、GNM1M2R61A105JNE17D、TZC3Z060A110R00 TZC3R100A110R00 TZV2R200A110 TZV2R030A110 TZV2Z06 0A110TZY2Z060A001 TZY2Z100A001 TZY2Z200A001电感常用料如下；LQG15HS1N5S02、LQG15HN15NJ02、LQG15HN18NJ02、LQG15HN3N9S02、LQG15HS5N6S02、LQG15HS6N8J02、LQP15MN8N2B02、LQP15MN4N7B02D、LQP15MN5N6B02D、LQP15MN27NJ02D、LQP18MN15NG02D、LQP18MN2N7C02D、LQP18MN3N3C02D、LQP18MN1N8C02、LQP18MN4N7C02D、LQP18MN27NG02D、LQH31MN100K03L、LQW15AN39NG00D、LQW15AN47NG00D、LQH43MN102K03L、LQW15AN5N6C10D、LQW15AN2N2C10D、磁珠常用料如下：BLM18HD102SN1D、BLM15BB750SN1D、BLM18BD252SN1D、BLM15BD182SN1D、BLM18PG221SN1D、BLM18HG601SN1D、BLM21AG121SN1D、BLM21PG221SN1D、BLM31PG330SN1L、BLM15HG601SN1D、BLM15AG121SN1D、BLM21BB331SN1D、BLM31PG601SN1L、BLM41PG600SN1L、BLM15BD102SN1D、BLM18HD102SN1D、热敏电阻常用料如下：NCP15WF104F03RC NCP21WB473J03RA NCP21XM472J03RA NCP21XW223J03RA NCP15XC220J03RC NCP15XW682J03RCNCP15XQ102J03RC NCP21XV103J03RA NCP15WB333J03RA NCP18XQ102J03R B NCP15XH103F03RC NCP18XH103F03RB陶瓷振荡子常用料如下：CSTCE16M0V53-R0、CSTCR4M00G53-R0、CSTCR6M00G53-R0、CSTLS20M0X53-B0、CSTCE18M4V53-R0、CSTCE8M00G52-R0、CSTLS4M00G53-B0、蓝牙滤波器常用料如下：LFB182G45SG9A293、LFB212G45BA1A220、LFB212G45SG8A192、声表滤波常用料如下：SAWEP942MCM0F00R12、SAFEA1G96FA0F00R12、SAFEA942MFA0F00、SAFEA881MAA0F00、SAFEA1G96AB0F00、SAFEA942MFL0F00R14、SAFEA1G84FA0F00R14、SAFEA881MFL0F00R14、SAWEN942MCM0F00R14、SAFEB1G57FM0F00、SAFEL1G96FA0F00R14、SAFEL1G84FA0F00R14、SAFEL942MFL0F00R14、SAFEL881MFL0F00R14滤波电容常用料号如下：NFM21PC105B1A3、NFM3DPC223R1H3L、NFE31PT221D1E9L、NFM18CC223R1C3D、NFM18PC105R0J3、NFM21PC474R1C3D、NFM3DCC101U1H3L、NFM41PC204F1H3L、NFM21PC104R1E3D、NFM21CC223R1H3D、NFM21PC224R1C3D、NFM3DCC471R1H3、NFM21CC222R1H3B、NFE31PT222Z1E9、NFE61PT101Z1H9L、NFE61PT472C1H9L、NFW31SP506X1E4、NFM41PC204F1H3、NFM41CC223R2A3L、NFM18PC104R1C3B、NFM18PC105R03J、BNX002-01共模扼流线圈常用料如下：DLW21SN900SQ2L、DLW21SN670SQ2L、DLW5BTN102SQ2L、DLP31SN221SL2、DLW5BTN142SQ2L、DLW5BSN152SQ2L、DLW5BSN191SQ2L、DLW5BTN101SQ2L、DLW5BSN302SQ2L、DLP31SN121ML2L、DLP11SN121SL2、DXW21BN7511T、DXP18BN5014TL射频元件常用料如下：射频测试线MXHS83QE3000 射频探头手机测试头MM126036 MM126038 同轴连接器 MM8430-2610 MM9329-2700天线开关常用料如下：LMSP33CA-465、LMSP33AA-696 、LMSP33AA-298、LMSP33QA-382、LMSP43MA-506联系人：朱先生手机：136******** QQ：1084623702 MSN：****************常用邮箱：*****************备用邮箱：****************公司地址：深圳市福田区上步南路国企大厦永富楼23F。

技术规格书
编号:
产品名称：磁珠
型号：RH 3.5*3*1.5
厂家：莆田市和达电子有限公司
供应商：厦门信和达电子有限公司
自年月日至年月日有效期：
自年月日至年月日
续签记录：
自年月日至年月日续签记录：
自年月日至年月日续签记录：
拟制：审核：批准：日期：
1、外观尺寸:
A、喷涂颜色正确，色彩一致，整体完整，边沿光滑，无毛刺、无裂纹、破损现象,
磁芯内部粉体没有结晶发亮现象，表面结晶总面积不得超过2mm2。

B、尺寸、喷涂颜色：
材质一经确认，生产工艺及材料配方不得做任何更改，若需更改，须征得我方同意。

3、电性能:(测试条件：ZL5 f=1KHz、U=1V)
3.1初始导磁率
以Φ0.25的漆包线密绕5匝，常温(25±2℃)放置2小时,测其电感量L
1
，要求：L1= 7-16uH
3.2居里温度
以Φ0.25的漆包线密绕5匝，
置于170℃下恒温半小时，测其电感量L
4，要求: L
4
≈0；
居里温度：160℃≤Tc≤175℃
4、包装
产品的内外包装(包括编带部分)应能达到防潮、抗震的作用,以防在运输或储存过程中产品受潮或挤压损坏等；内外包装标识应正确清楚。

内外包装标识应包括产品型号、规格、生产日期、生产批号、保质期（有效使用期）、检验日期、数量等。

磁珠选型参数1. 简介磁珠是一种常用的生物分离和纯化技术，广泛应用于生物医学研究、临床诊断和生产制造等领域。

磁珠选型参数是指在使用磁珠进行分离和纯化时，需要考虑的与磁珠性能相关的参数。

本文将详细介绍磁珠选型参数的相关内容。

2. 磁珠选择在选择合适的磁珠时，需要考虑以下几个关键参数：2.1 粒径磁珠的粒径是指其直径大小，通常以纳米为单位表示。

粒径的选择取决于待分离物的大小和所需纯度。

一般而言，较小的粒径能提供更高的分辨率和更好的纯度，但可能会降低操作效率。

大多数应用中常用的磁珠粒径为50-200纳米。

2.2 表面修饰磁珠表面通常会进行修饰以增加其亲和性或特定功能。

例如，可以将氨基酸、抗体、核酸等物质固定在磁珠表面，以实现对特定分子的选择性结合。

选择合适的表面修饰可以提高磁珠的选择性和纯度。

2.3 磁性磁珠的磁性是指其对外加磁场的响应能力。

高磁性的磁珠具有较强的吸附能力和迅速的分离速度，但也可能对待分离物造成较大的机械剪切力。

低磁性的磁珠则具有较弱的吸附能力和较慢的分离速度，但对待分离物影响较小。

根据实际需求，选择适当磁性的磁珠是非常重要的。

2.4 稳定性在使用过程中，磁珠需要保持良好的稳定性，不发生聚集、沉淀或颗粒损失等现象。

因此，选择具有良好稳定性且耐受多次反复洗涤、重悬和储存处理的磁珠是必要的。

3. 磁珠选型参数影响因素在确定合适的磁珠选型参数时，需要考虑以下几个主要影响因素：3.1 待分离物特性待分离物的特性对磁珠选型参数有直接影响。

例如，如果待分离物是蛋白质，可以选择具有亲和基团的磁珠；如果待分离物是核酸，可以选择具有亲和碱基或磷酸基团的磁珠。

3.2 样品来源和性质样品来源和性质也会对磁珠选型参数产生影响。

例如，如果样品是血液、组织或细胞等复杂样品，可能需要选择具有更高选择性和较大表面积的磁珠。

3.3 分离纯度要求不同的应用对分离纯度有不同的要求。

某些应用可能对纯度要求较高，需要选择具有更好选择性和较小粒径的磁珠；而其他应用则对纯度要求相对较低。

链霉亲和素磁珠使用说明货号：S7210规格：1mL（10mg/mL）保存：2-8℃产品内容：Beads Mag SA磁珠是采用定向固定技术将重组中性链霉亲和素共价偶联到形态规整、粒径均一的磁性微球上，形成单分子固定层，可用于生物素化核酸、抗体或其他生物素化配体和靶分子的分离和检测。

由于具有单层的链霉亲和素，绝大多数生物素结合位点在空间上不仅可以结合游离生物素，而且还可以结合生物素化的配体/靶标，具有快速液相反应动力学特性。

形状确定的特异性表面便于进行高效捕获、分离和下游操作，链霉亲和素单层可确保没有明显泄漏，而通过避免吸附过量的链霉亲和素，批次一致性和结果的可重复性得到了保证。

Beads Mag SA以聚合物为基材的实心微球，主要用于免疫检测、免疫沉淀、细胞分选等。

产品特性：产品名称Beads Mag SA基质Polymer粒径2μm浓度10mg/ml保存条件PBST(pH7.4,0.01%Tween-20)，2-8℃结合量1000pmol free biotin/mg of beads20μg biotinylated antibody/mg of beads400pmol biotinylated oligonucleotides/mg of beads注意事项：1.请勿离心、干燥或者冷冻磁珠，这些操作可能导致磁珠的聚集从而降低结合活性；2.从磁珠保存管中移取磁珠前应充分震荡重悬均匀，操作过程中应避免产生气泡；3.生物素标记好蛋白或核酸后，用脱盐柱去掉多余的游离生物素；4.尽量减少蛋白降解，包括制备细胞裂解液中包含的蛋白酶抑制剂；5.生物素化分子的大小会影响磁珠的载量，用户需要根据实验确定磁珠对特定生物素化分子的载量。

手动操作步骤：以下操作过程需要准备的试剂：注：用户可根据需要调整缓冲液的盐浓度及pH1.固定化核酸1.1将磁珠瓶置于漩涡振荡器上20s，振荡重悬磁珠，取100μl 磁珠到新的离心管中，置于缓冲液名称成分Buffer I（适用于结合生物素化核酸）10mM Tris-HCl（pH7.5），1mM EDTA，1M NaCl ，0.01%~0.1%Tween-20Buffer II （适用于结合生物素化抗体/蛋白）PBS，pH7.4，含0.05%Tween-20，可根据需要添加0.01%~0.1%BSA磁力架上，1min后移除上清液；注意：用户可根据生物素化分子的多少，参考磁珠的载量，计算需要取用的磁珠量，建议生物素化分子的加入量为磁珠载量的1~2倍，使磁珠饱和。

版本2022/09/08（02）
链霉亲和素纳米磁珠（100-300nm ）说明书1/1链霉亲和素纳米磁珠（100-300nm ）产品说明书
【产品名称】链霉亲和素纳米磁珠（100-300nm ）
【英文名称】Streptavidin Nano Magnetic Beads (100-300nm)
【订货信息】
纳米磁珠/纯水【简介】
东纳生物科技有限公司提供链霉亲和素纳米磁珠（100-300nm ），链霉亲和素磁珠可与生物素化的多肽、蛋白、抗体等生物配体高效偶联，应用于免疫分析、基因分析和纯化PCR 产物等。

【产品参数】
图1：100nm 链霉亲和素磁珠扫描电镜（左图，100±10nm ）、200nm 链霉亲和素磁珠扫描电镜（中图，
220±30nm ）以及300nm 链霉亲和素磁珠扫描电镜（右图，310±20nm ）。

【注意事项】
1.磁珠取用前应充分混匀，防止取用改变磁珠浓度，避免长时间超声对磁珠表面破坏；
2.磁珠取用后，使用前请进行磁分离并用纯水或所用缓冲溶液清洗2-3遍；
3.磁珠使用和保存过程中应避免冻融。

【生产单位】
公司名称
南京东纳生物科技有限公司地址
南京市江宁区龙眠大道568号南京生命科技小镇5号楼北楼6楼邮政编码
210000电话号码
025********电子邮箱
**************公司网站。

Contents1. Description1.1 Principle of the MACS® Separation1.2 Background information1.3 Applications1.4 Reagent and instrument requirements试剂和仪器的要求2. Protocol2.1 Sample preparation样品制备2.2 Magnetic labeling磁性标记2.3 Magnetic separation磁性分离3. Example of a separation using the CD133 MicroBead Kit4. References1. DescriptionComponents 2 mL CD133 MicroBeads, human:MicroBeads conjugated to monoclonal antihumanCD133 antibodies (isotype: mouse IgG1,clone AC133).2 mL FcR Blocking Reagent, human Specificity CD133 antigen, epitope (CD133/1)1.Capacity For 2亊10⁹total cells, up to 100 separations.Product format CD133 MicroBeads are supplied in buffercontaining stabilizer and 0.05% sodium azide.Storage Store protected from light at 2−8 °C. Do not freeze. The expiration date is indicated on the vial label.1.1 Principle of the MACS® SeparationFirst, the CD133+ cells are magnetically labeled with CD133MicroBeads. Then, the cell suspension is loaded onto a MACS®Column, which is placed in the magnetic field of a MACS Separator.The magnetically labeled CD133+ cells are retained within thecolumn. The unlabeled cells run through; this cell fraction isthus depleted of CD133+ cells. After removing the column fromthe magnetic field, the magnetically retained CD133+ cells can beeluted as the positively selected cell fraction. To increase the purity,the positively selected cell fraction containing the CD133+ cells isseparated over a second column.1.2 Background informationThe CD133 MicroBead Kit is a magnetic labeling system designedfor the positive selection of CD133+ cells. It allows the single-stepisolation of nonhematopoietic and early hematopoietic progenitors and stem cells. The CD133 molecule is a 5-transmembrane cellsurface antigen with a molecular weight of 117 kD.2 The CD133/1(clone AC133) antibody recognizes epitope 1 of the CD133 antigen.1In the hematopoietic system, CD133 expression is restricted to asubset of CD34bright stem and progenitor cells in human fetal liver,bone marrow, cord blood, and peripheral blood.3 Isolated fromhematopoietic sources, CD133+ cells can become adherent and arereported to become CD133–during culture⁴. The CD34+CD133+cell population, which includes CD34+CD38–cells, was shown tobe capable of repopulating NOD/SCID mice.⁵Recently, CD133has also been found to be expressed on circulating endothelialprogenitor cells⁶,⁷and fetal neural stem cells⁸,⁹as well as on othertissue-specific stem cells, such as renal1⁰and prostate11 stem cells.Lately, when isolated from tumor tissue, the CD133+ populationcan be enriched for tumor-initiating cells.11-1⁵CD133 MicroBeadshave been used to isolate adult stem cells from cord blood and asa starting population for reprograming towards iPS cells.1⁶CD133expression has been found on undifferentiated human ES cells.Therefore CD133 MicroBeads could be used for enrichment ordepletion of these cells.1⁷1.3 Applications●Positive selection or depletion of cells expressing human CD133antigen.●Isolation or depletion of CD133+ cells from peripheral bloodmononuclear cells (PBMCs) or single-cell suspensions fromtissue.●CD133+ cells are used in basic stem cell research, stem cellevaluation, stem cell expansion, research in hematologicalmalignancies, stem cell plasticity, and potential cellulartherapies as well as in tissue regeneration and cancer research.1.4 Reagent and instrument requirements●Buffer: Prepare a solution containing phosphate-buffered saline(PBS), pH 7.2, 0.5% bovine serum albumin (BSA), and 2 mMEDTA by diluting MACS BSA Stock Solution (# 130‑091-376)1:20 with autoMACS Rinsing Solution (# 130-091-222). Keepbuffer cold (2−8 °C). Degas buffer before use, as air bubblescould block the column.▲Note: EDTA can be replaced by other supplements such as anticoagulant citrate dextrose formula-A (ACD-A) or citrate phosphate dextrose (CPD). BSA can be replaced by other proteins such as human serum albumin, human serum, or fetal bovine serum (FBS). Buffers or media containing Ca2+ or Mg2+ are not recommended for use.●(Optional) Fluorochrome-conjugated antibodies forflow cytometric analysis, e.g., CD133/2 (293C3)-PE(# 130-090-853), CD133/2 (293C3)-APC (# 130-090-854),CD133/2 (293C3)‑Biotin, CD34-FITC (# 130-081-001),CD34‑APC (# 130-090-954), or CD34-PE (# 130-081-002). Formore information about fluorochrome-conjugated antibodiessee .●MACS Columns and MACS Separators: CD133+ cells can beEnriched浓缩by using MS, LS, or XS Columns or depleted withthe use of LD, CS, or D Columns. Cells which strongly expressthe CD133 antigen can also be depleted using MS, LS, or XSColumns. Positive selection正向or depletion can also be performedby using the autoMACS Pro or the autoMACS Separator.▲Note: Column adapters are required to insert certain columns into theV arioMACS™or SuperMACS™Separators. For details see the respective MACS Separator data sheet.●(Optional) Propidium Iodide Solution (# 130-093-233) or7-AAD for flow cytometric exclusion of dead cells.●(Optional) Dead Cell Removal Kit (# 130-090-101) for thedepletion of dead cells.●(Optional) Pre-Separation Filters (# 130-041-407) to removecell clumps团.2. Protocol2.1 Sample preparationWhen working with anticoagulated peripheral blood or buffy coat,peripheral blood mononuclear cells (PBMCs) should be isolated bydensity gradient centrifugation, for example, using Ficoll-Paque™.▲Note: To remove platelets after density gradient separation, resuspend cell pellet in buffer and centrifuge at 200×g for 10−15 minutes at 20 °C. Carefully aspirate supernatant. Repeat washing step.When working with tissues or lysed blood, prepare a single-cellsuspension using standard methods.For details see the protocols section at /protocols.For preparation of cord blood cells, bone marrow cells, or cellsfrom leukapheresis material, please refer to the sample preparationprotocols at /protocols.▲Dead cells may bind non-specifically to MACS MicroBeads.To remove dead cells, we recommend using density gradientcentrifugation or the Dead Cell Removal Kit (# 130-090-101).2.2 Magnetic labeling▲Work fast, keep cells cold, and use pre-cooled solutions. This willprevent capping of antibodies on the cell surface and non-specificcell labeling.▲V olumes for magnetic labeling given below are for up to10⁸total cells. When working with fewer than 10⁸cells, use the same volumes as indicated. When working with higher cell numbers,scale up all reagent volumes and total volumes accordingly (e.g.for 2亊10⁸total cells, use twice the volume of all indicated reagent volumes and total volumes).▲For optimal performance it is important to obtain a single‑cell suspension before magnetic labeling. Pass cells through 30 μm nylonmesh (Pre-Separation Filters, # 130-041-407) to remove cell clumpswhich may clog the column. Moisten filter with buffer before use.▲The recommended incubation temperature is 2–8 °C. Workingon ice may require increased incubation times. Higher temperaturesand/or longer incubation times may lead to non-specific celllabeling.1. Determine确定cell number.2. Centrifuge cell suspension细胞悬液at 300×g for 10 minutes. Aspirate supernatant completely.吸取上清3. Resuspend cell pellet in 300 μL of buffer per 10⁸total cells.4. Add 100 μL of FcR Blocking Reagent per 10⁸total cells.5. Add 100 μL of CD133 MicroBeads per 10⁸total cells.6. Mix well and incubate for 30 minutes in the refrigerator(2−8 °C).7. (Optional) Add staining antibodies, e.g., 50 μL of CD133/2(293C3)-PE (# 130-090-853), and incubate for 5 minutes in thedark in the refrigerator (2−8 °C).8. Wash cells by adding 1−2 mL of buffer per 10⁸cells andcentrifuge at 300×g for 10 minutes. Aspirate supernatantcompletely.9. Resuspend up to 10⁸cells in 500 μL of buffer.▲Note: For higher cell numbers, scale up buffer volume accordingly.▲Note: For depletion with LD Columns, resuspend up to 1.25亊10⁸cells in 500 μL of buffer.10. Proceed to magnetic separation (2.3).2.3 Magnetic separation▲Choose an appropriate MACS Column and MACS Separatoraccording to the number of total cells and the number of CD133+cells. For details see table in section 1.4.▲Always wait until the column reservoir is empty before proceedingto the next step.Magnetic separation with MS or LS Columns▲To achieve highest purities, perform two consecutive columnruns.1. Place column in the magnetic field of a suitable MACS Separator.For details see the respective MACS Column data sheet.2. Prepare column by rinsing with the appropriate amount ofbuffer:MS: 500 μL LS: 3 mL3. Apply cell suspension onto the column. Collect flow-throughcontaining unlabeled cells.4. Wash column with the appropriate amount of buffer. Collectunlabeled cells that pass through and combine with the effluentfrom step 3.MS: 3×500 μL LS: 3×3 mL▲Note: Perform washing steps by adding buffer aliquots only when the column reservoir is empty.5. Remove column from the separator and place it on a suitablecollection tube.▲Note: To perform a second column run, you may elute the cells directly from the first onto the second, equilibrated column instead of a collection tube.6. Pipette the appropriate amount of buffer onto the column.Immediately flush out the magnetically labeled cells by firmlypushing the plunger into the column.MS: 1 mL LS: 5 mL7. To increase purity of CD133+ cells, enrich the eluted fractionover a second MS or LS Column. Repeat the magneticseparation procedure as described in steps 1 to 6 by using anew column.Magnetic separation with XS ColumnsFor instructions on the column assembly and the separation refer tothe XS Column data sheet.Depletion with LD Columns1. Place LD Column in the magnetic field of a suitable MACSSeparator. For details see LD Column data sheet.2. Prepare column by rinsing with 2 mL of buffer.3. Apply cell suspension onto the column.4. Collect unlabeled cells that pass through and washcolumn with 2×1 mL of buffer. Collect total effluent;this is the unlabeled cell fraction. Perform washingsteps by adding buffer two times. Only add new buffer whenthe column reservoir is empty.Depletion with CS Columns1. Assemble CS Column and place it in the magnetic field of asuitable MACS Separator. For details see CS Column datasheet.2. Prepare column by filling and rinsing with 60 mL of buffer.Attach a 22G flow resistor to the 3-way stopcock of theassembled column. For details see CS Column data sheet.3. Apply cell suspension onto the column.4. Collect unlabeled cells that pass through and wash columnwith 30 mL buffer from the top. Collect total effluent; this isthe unlabeled cell fraction.Depletion with D ColumnsFor instructions on column assembly and separation refer to theD Column data sheet.Magnetic separation with the autoMACS® Pro Separator or theautoMACS® Separator▲Refer to the respective user manual for instructions on how to use the autoMACS Pro Separator or the autoMACS Separator.▲Buffers used for operating the autoMACS Pro Separator or the autoMACS Separator should have a temperature of ≥10 °C.▲Program choice depends on the isolation strategy, the strengthof magnetic labeling, and the frequency of magnetically labeled cells. For details refer to the section describing the cell separation programs in the respective user manual.Magnetic separation with the autoMACS® Pro Separator1. Prepare and prime the instrument.2. Apply tube containing the sample and provide tubes for collecting the labeled and unlabeled cell fractions. Placesample tube in row A of the tube rack and the fractioncollection tubes in rows B and C.3. For a standard separation choose one of the following programs:Positive selection from peripheral blood, bone marrow, or leukapheresis: “Posseld”Collect positive fraction in row C of the tube rack.Positive selection from cord blood: “Posseld2”Collect positive fraction in row C of the tube rack.Depletion: “Depletes”Collect negative fraction in row B of the tube rack.Magnetic separation with the autoMACS® Separator1. Prepare and prime the instrument.2. Apply tube containing the sample and provide tubes for collecting the labeled and unlabeled cell fractions. Placesample tube at the uptake port and the fraction collectiontubes at port neg1 and port pos 2.3. For a standard separation choose one of the following programs:Positive selection from peripheral blood, bone marrow, or leukapheresis: “Posseld”Collect positive fraction from outlet port pos 2.Positive selection from cord blood: “Posseld2”Collect positive fraction from outlet port pos 2.Depletion: “Depletes”Collect negative fraction from outlet port neg1.3. Example of a separation using the CD133MicroBead KitCD133+ hematopoietic stem and progenitor cells were isolated from non-mobilized human PBMCs using the CD133 MicroBead Kit, MS Columns, and a MiniMACS™Separator. Cells were fluorescently stained with CD34-FITC (# 130-081-001) and CD133/2 (293C3)-PE (# 130-090-853) and analyzed by flow cytometry. Cell debris and dead cells werde excluded from the analysis based on scatter signals and propidium iodide fluorescence.All protocols and data sheets are available at .WarningsReagents contain sodium azide. Under acidic conditions sodium azide yields hydrazoic acid, which is extremely toxic. Azide compounds should be diluted with running water before discarding. These precautions are recommended to avoid deposits in plumbing where explosive conditions may develop.WarrantyThe products sold hereunder are warranted only to be free from defects in workmanship and material at the time of delivery to the customer. Miltenyi Biotec GmbHmakes no warranty or representation, either expressed or implied, with respect tothe fitness of a product for a particular purpose. There are no warranties, expressedor implied, which extend beyond the technical specifications of the products.Miltenyi Biotec GmbH’s liability is limited to either replacement of the products or refund of the purchase price. Miltenyi Biotec GmbH is not liable for any property damage, personal injury or economic loss caused by the product.autoMACS and MACS are registered trademarks and MidiMACS, MiniMACS, OctoMACS, QuadroMACS, SuperMACS, and V arioMACS are trademarks of Miltenyi Biotec GmbH.Ficoll-Paque is a trademark of GE Healthcare companies.Copyright . 2009 Miltenyi Biotec GmbH. All rights reserved.。

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