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GoldBio/Agarose LE (Molecular Biology Grade)/100 g/A-201-100
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GoldBio/Agarose LE (Molecular Biology Grade)/100 g/A-201-100
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A-201-100
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Agarose LE (Low Electroendosmosis) is Molecular Biology Grade and is specifically designed for the superior separation of nucleic acids, with maximally crisp band resolution, and is also ideal for cloning and cloning related experiments.

GoldBio Agarose LE is refined in an advanced process that excludes the use of organic solvents. The result is a cleaner end-product with significantly reduced environmental impact. The agarose can be used for analyses of nucleic acids from 50 bp to 25 kbp, protein electrophoresis and various blotting protocols.

The low EEO of the agarose promotes increased electrophoretic mobility, yielding improved resolution and shorter run times. This also allows macromolecules and larger particles (subcellular fragments, viruses, etc.) to migrate more freely through the gel matrix. The consistently low EEO reduces band distortion (caused by counterflow) that can result from the presence of excessive sulfate-rich negative ions.

Agarose is a natural product that forms an inert matrix used in electrophoresis, chromatography and other molecular biology and biochemistry techniques. Likewise, it is neutral and easily derivatizable, so it is easy to bind to its structure proteins like enzymes, antigens or antibodies. Toxicity absence makes working with agarose very convenient.

Agarose LE Gel Applications:

  • Gel electrophoresis
  • Nucleic acid analytical and preparative electrophoresis
  • High electrophoresis mobility
  • Blotting assays
  • Protein electrophoresis such as radial immunodiffusion

Technical Specifications

Agarose LE

Molecular Biology Grade

EEO (Electroendomosis): ≤0.12Sulfate: ≤0.1%Gel Strength (1%): ≥1200 g/cm 2Gelling Temperature: 36±1.5°CMelting Temperature: 88±1.5°CDNase/RNase Activity: None DetectedDNA Resolution ≥1000 bp: Finely ResolvedGel Background: Very LowDNA Binding: Very Low

Agarose LE Features:

  • Extraordinary mechanical resistance for more reliable andeasier handling
  • Excellent transparency of the gel and high visibility
  • Possibility of varying pore size in accordance with particle sizeby modifying the gel concentration
  • Absence of toxicity (polyacrylamide is neurotoxic)
  • Easy preparation of the gel by simple dilution in aqueousbuffers either by standard boiling or microwaving
  • Greater thermal stability due to high hysteresis (differencebetween gelling and melting temperatures)

Which agarose gel type should I choose?

Below is a table to help you choose which agarose gel type is suited for your experimental needs.

Bases

Agarose Type

<1 kb

High Resolution Agarose

50 bp – 25 kbp

Agarose LE

>1000 bp

Low Melt Agarose

Agarose volume chart

The volume needed for your agarose gel depends on the size of your gel casting tray. Mini gels carried out on small trays use 40 mL agarose gel. The table below shows agarose gel tray dimensions and a corresponding volume range.

Gel Tray Dimensions (cm)

Agarose Gel Volume Range

7 x 8 cm

40 ml

9 x 11 cm

70 – 80 ml

12 x 14 cm

120 – 130 ml

Agarose LE Quick Answers:

What is an agarose gel?

What does LE in Agarose LE Mean?

What is agarose used for?

How do you prepare agarose gel/ How do you dissolve agarose?

What percent agarose gel should I use?

How do I reuse or remelt agarose gel?

What is an agarose gel?

Agarose is a polysaccharide that comes from red seaweed and has been processed in such a way that agaropectin has been removed. In molecular biology, this separated product, known as agarose, is used to separate fragments of DNA in a process called gel electrophoresis.

The molecular composition of agarose, which sort of resembles a mesh or net, helps slow down the movement of DNA to where smaller fragments travel through the agarose gel quicker, and larger fragments travel through the agarose gel slower.

Pictured below is a rendering of how an agarose gel might look at the molecular level. To the naked eye, an agarose gel looks like a clear, gelatin material. However, at the molecular level, an agarose gel resembles more of a porous substance or mesh. The second figure is an illustration that shows how smaller molecules would easily travel through the mesh-like makeup of agarose gel, whereas larger molecules will get caught and travel slowly.

Agarose LE Gel matrix agarose gel

Illustration of DNA traveling through an agarose gel at the molecular level. This illustration shows the porous makeup of agarose LE and how the mesh-like matrix separate smaller DNA fragments from larger DNA fragments.

During a specific period in which the agarose gel is run, researchers will be able to distinguish larger fragments of DNA from smaller fragments of DNA by looking at how far down the agarose gel their sample moved. Those bands closest to the well, which have not moved very far, are larger fragments of DNA. By using a molecular weight marker or DNA ladder, researchers are able to measure their DNA fragment sample against a standard ladder of different DNA fragments.

Illustration of an agarose gel with a DNA ladder and 3 lanes. The first lane has a large fragment that did not move far down the agarose gel while in the next lane a smaller fragment has moved further down the agarose gel

What does LE in Agarose LE Mean?

The LE in Agarose LE stands for Low EEO or low electroendosmosis, which describes the electrically influenced movement of material through porous material. A low EEO, or using Agarose LE will increase mobility, reduce band distortion that is caused by counter flow, and provide better resolution. Low EEO Agarose also allows larger particles such as viruses to migrate within the matrix.

What is agarose used for?

Agarose gels are used in a method called gel electrophoresis, which electrically separates DNA fragments based on size, allowing researchers to determine their specific DNA fragment.

Agarose LE Gel Applications Include:

  • Gel electrophoresis
  • Nucleic acid analytical and preparative electrophoresis
  • High electrophoresis mobility
  • Blotting assays
  • Protein electrophoresis such as radial immunodiffusion

Because the structure of an agarose gel, at the molecular level, is a matrix and porous, larger DNA fragments travel slowly through the gel, while smaller fragments travel quickly and therefore farther down the gel. These bands of DNA can be compared against a DNA ladder, allowing researchers to determine size.

Furthermore, understanding DNA fragment size, helps researchers validate their sample of interest. A simple example would be if a researcher knows they are looking specifically for a sample that is 1500 kilobases, but perhaps have five tubes with five different samples, the researcher can run them on an agarose gel, and then compare the samples and sizes.

How do you prepare agarose gel/ How do you dissolve agarose?

You can dissolve and prepare your agarose gel with these steps:

  • Determine the concentration needed for your agarose gel.
  • Measure out the required mass of agarose LE powder.
  • Add the required volume of diluted TAE buffer to a flask that holds 2-4 times the volume needed for your agarose gel.
  • Add your measured agarose powder to your flask.
  • Use a magnetic stir bar to mix the solution.
  • Once the solution is mixed, remove the stir bar. Place the flask in a lab microwave with a loose lid over the flask or cover the flask with plastic wrap (vent the plastic wrap with a hole).
  • Heat the flask in the microwave in bursts of 30 seconds. Swirl your agarose mixture after each burst.
  • Once the agarose powder is fully dissolved and the liquid appears clear, allow it to cool until it’s safe to touch with your bare hands.
  • Once it is cooled, you can pour your agarose gel mixture into the gel mold with comb. Wait for the gel to cool until it solidifies.
  • Gently remove the comb once your gel is cooled and solidified. Then you can load your DNA.

What percent agarose gel should I use?

The percent agarose gel used for electrophoresis depends on the size of DNA you’re working with. Below is a table showing what percent gel to use based on your DNA size.

Concentration (%)

DNA Size Resolution (bp)

0.5

1,000 – 25,000

0.75

800 – 12,000

1.0

500 – 10,000

1.2

400 – 7,500

1.5

200 – 3,000

2.0

50 – 1,500

How do I reuse or remelt agarose gel?

An agarose gel can be reused by remelting the gel in the laboratory microwave. This helps save some money. However, it is not always advantageous to reuse your agarose gel.

remelt and reuse your agarose gel when your

Reuse your agarose gel when:

You’re just running routine gels or doing a demonstration.

do not remelt or reuse your agarose gel to confirm findings, publish your results, cloning, sequencing, doing an extraction, doing a Southern blot, or doing more polished work. In these cases, it’s always best to make a fresh agarose gel.

It’s best not to reuse your agarose gel when:

You’re confirming findings, publishing results, cloning, sequencing, doing extractions, doing a Southern blot, or for polished work. Instead make a fresh agarose gel.

GoldBio活体成像技术:早在1999年由美国哈佛大学Weissleder博士率先提出了分子影像学(molecularimaging,MI)的概念,即应用影像学的方法对活体状态下的生物过程进行细胞和分子水平的定性和定量研究。活体成像便是基于分子影像学孕育而生的,通过这个成像系统,可以观测活体动物体内肿瘤的生长及转移,感染性疾病的发展进程,特定基因的表达等生物学过程。活体成像技术主要采用生物发光(bioluminescence)与荧光(fluorescence)两种技术。★生物发光是用荧光素酶基因标记细胞或DNA。★荧光技术则采用荧光报告基团(GFP、RFP,Cyt及dyes等)进行标记。★这一技术对肿瘤微小转移灶的检测灵敏度极高,不涉及放射性物质和方法,非常安全。操作极其简单、所得结果直观、灵敏度高。


活体成像两种检测技术介绍活体成像特点优点缺点生物发光检测bioluminescence★荧光素酶(Luciferase)对基因、细胞和活体动物进行标记;★荧光素酶催化底物(例如荧光素钾盐)反应后,会产生化学发光。这种光是由化学反应而来,不需要激发光;★标记方法是通过克隆技术,将荧光素酶的基因插入到预期观察的细胞染色体内,通过对克隆细胞进行筛选,培养出能稳定表达荧光素酶的细胞株。再将细胞株转移至特定的小鼠体内形成模型。★特异性强,无自发荧光;★高灵敏度,在体内可检测到几百个细胞,检测的深度在3-100px;★定量精确 ★信号较弱,检测时间较长;★仪器精密度要求较高;★细胞或基因需要转基因标记;★不可用于人体,不适用于抗体多肽等标记荧光检测fluorescence★采用荧光报告基因(GFP、RFP等)或荧光染料进行标记;★需要外接激发光源,利用报告基因、荧光蛋白质或染料产生的荧光,就可以形成体内的生物光源。★荧光染料、蛋白标记能力强;★信号强,成像速度快,操作简便,实验成本较低;★未来可用于人;★适用范围广,可以是动物、细胞、微生物,也可以是抗体、药物、纳米材料等。★存在自发荧光,影响灵敏度;★光容易被动物组织吸收;★检测深度受限;★背景光干扰,定量准确度低



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商品咨询

请问下有无同学需要H37RA的?我是做EAE模型的,上个月购买了BDDifco公司的H37RA(货号),因为购买的时候只能整盒6支购买,但我们用不了那么多,所以想问问有无同学需要的,100mg/支,800元/支或用等价试剂交换。地址广州。有需要的请私信,谢谢!

最近发现一个问题一般生化仪至少能检测二三十个项目!那么问题是这么多项目要加的试剂R1,R2,算下来也得六七十个瓶瓶罐罐,每天加试剂,倒过来倒过去的,很容易把试剂加错吧?所以就想问一下各位平时工作中有......
下列各种溶液,不用其它试剂就能鉴别的是()
A、Na2CO3HClH2SO4NaNO3
B、K2CO3H2SO4HNO3BaCl2
C、HClHNO3AgNO3NaCl
D、NaOHFeCl3MgCl2BaCl2

我想检测血管组织中的钙离子浓度,不知道哪个公司有试剂盒

只用胶头滴管和试管,不用其他试剂就可以区别的下列溶液(浓度均为)是(   )A.和B.稀和C.和D.和盐酸

我们做体外诊断仪器,打算购买别人的试剂灌装到我们设计的芯片中使用(耗材)。请问几个问题,1,试剂是否需要注册。2,生产、技术、质量相关人员是否需要专业要求。3灌装是否需要在洁净室生产

盐酸和乙醛能和氢氧化铜反应,乙醇不反应。所以两两混合。
1.KOH,Na2SO4,AlCL3
2.NaHCO3,Ba(OH)3,H2SO4
3.HCL,NaAlO2,NaHSO4
4.Ca(OH)2,Na2CO3,BaCO3
谢谢了
要原因
anaohna2co3nahco3ba(oh)2
bhclna2so4nano3na2co3
chclnaohna2co3nacl
dba(oh)2nahco3alcl3nahso4
乙醇,乙醛,盐酸,CU(OH)2悬浊液
A.KOH溶液和AlCl3溶液B.Na2CO3溶液和盐酸
C.MgCl2溶液和氨水D.盐酸和NaAlO2溶液
为什么

求购上图结构的N-保护的三氨基丙烷衍生物,以及荧光染料BODIPY和铂试剂。主要是该结构化合物或者合成该化合物的前体