FlexiTube siRNA

每次对单个基因进行高效RNAi分析

Products

FlexiTube siRNA 旨在用于分子生物学应用。该产品不能用于疾病诊断、预防和治疗。
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FlexiTube GeneSolution

Cat. No. / ID:   1027416

siRNA GeneSolution details
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FlexiTube siRNA (20 nmol)

Cat. No. / ID:   1027419

20 nmol siRNA with modification options delivered in tubes
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FlexiTube siRNA (20 nmol)

Cat. No. / ID:   1027418

20 nmol siRNA delivered in tubes
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FlexiTube siRNA (5 nmol)

Cat. No. / ID:   1027417

5 nmol siRNA delivered in tubes
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FlexiTube siRNA (1 nmol)

Cat. No. / ID:   1027415

1 nmol siRNA delivered in tubes

特点

  • 经济高效的siRNA,方便分析更多基因
  • 为每个基因优化的方案
  • 创新的设计最大可能减小脱靶效应
  • 在GeneGlobe可方便的检索并订购siRNA

产品详情

FlexiTube siRNA可对少量基因进行经济高效的RNAi分析。人类、小鼠和大鼠基因的siRNA提供5 nmol或20 nmol两种规格,对于人类和小鼠基因还有更经济的1 nmol规格可供选择。

FlexiTube GeneSolution含有4条预选的siRNA,用于特定靶基因(各1 nmol)。FlexiTube GeneSolution使用多个siRNA研究一个靶基因,确保结果的可靠性。FlexiTube siRNA和FlexiTube GeneSolution使用创新的HP OnGuard siRNA设计,详情请参见QIAGEN GeneGlobe。

绩效

性能保证

FlexiTube siRNA承诺提供一次性更换。如果订购了同一靶基因的多条FlexiTube siRNA,且至少2条未表现≥70%的基因抑制,QIAGEN将提供2条免费的额外siRNA,仅限一次。用户需要提供支持数据,以证明在适宜的转染条件下,siRNA未能成功地在mRNA水平抑制≥70%的靶基因。支持数据需要包括转染率数据,定量沉默数据以及≥70%的阳性对照抑制数据。该承诺自发货之日起6个月内有效。

数千条实验验证的siRNA

数千条人类siRNA已经通过real-time RT-PCR验证,表现出至少70%的基因抑制。关于这些siRNA验证实验的详细信息和抑制水平信息,请参见GeneGlobe网站。这些经验证的siRNA均来自由QIAGEN科学家完成的世界最大规模的siRNA验证项目。如需该项目更多信息,请参见Krueger, U. et al. (2007) Insights into Effective RNAi Gained from Large-Scale siRNA Validation Screening. Oligonucleotides 17, 237.

领先的siRNA设计

QIAGEN在siRNA设计中的进步性,确保其高度创新且精良的HP OnGuard siRNA Design,能提供高效特异的siRNA。根据来自RNAi试验的数据建立极大容量的数据库,并在此基础上利用神经网络技术进行siRNAs设计,然后使用先进的、非冗余序列数据库和同源分析工具,检查该序列与同一基因组内其他序列的同源性。HP OnGuard siRNA Design具有许多独特先进的特性(见下表)。

HP OnGuard siRNA Design特性
特性描述 参考
神经网络技术 使用BioPredsi神经网络设计siRNA,依托于极大的RNAi数据库。 1-3
全球最大的siRNA验证项目 该项目提供的数据使设计过程更完善,QIAGEN科学家已通过成千上万的siRNA确认其效能。该项目证实大量药用基因组siRNA功能至少有70%可被抑制。 4
同源性分析 该分析使用专用工具以及最新的,非冗余序列数据库。
Affymetrix基因芯片分析 基因组范围siRNA设计的创新性发展最大程度减少脱靶效应。
最新的siRNA靶序列 NCBI数据库的最新数据确保设计的准确性。
不对称性 对siRNA的设计基于5’端碱基对的不等稳定性,使得有义链被降解的同时,反义链在5’端的结合度降低而进入RISC。利用不对称性可制备高度可用的siRNA,且大大降低了错误链进入RISC而导致脱靶效应的风险。 5, 6
3' UTR/seed区域分析 使用智能加权分析,多参数搜索与非目的靶标mRNA3’非编码区相匹配的siRNA反义链的源区域。 7-12
SNP位点屏蔽 采用RefSNP数据库排除单核苷酸多态(SNP)的siRNA,由于这种siRNA有效性不同从而提高了siRNA的效果。
干扰素序列屏蔽 屏蔽掉可导致干扰素反应的多重序列基序siRNA,弃用含有这种基序的siRNA。 13, 14
1. Huesken, D. et al. (2005) Design of a genome-wide siRNA library using an artificial neural network. Nat. Biotechnol. 23, 995.
2. Mukherji, M. et al. (2006) Genome-wide functional analysis of human cell-cycle regulators. Proc. Natl. Acad. Sci. 103, 14819.
3. Matveeva, O. et al. (2007) Comparison of approaches for rational siRNA design leading to a new efficient and transparent method. Nucleic Acids Res. 35, e63.
4. Krueger, U. et al. (2007) Insights into effective RNAi gained from large-scale siRNA validation screening. Oligonucleotides 17, 237.
5. Aza-Blanc, P. et al. (2003) Identification of modulators of TRAIL-induced apoptosis via RNAi-based phenotypic screening. Mol. Cell 12, 627.
6. Schwarz, D.S. et al. (2003) Asymmetry in the assembly of the RNAi enzyme complex. Cell 115, 199.
7. Farh, K.K. et al. (2005) The widespread impact of mammalian microRNAs on mRNA repression and evolution. Science 310, 1817.
8. Grimson, A. et al. (2007) MicroRNA targeting specificity in mammals: determinants beyond seed pairing. Mol. Cell 27, 91.
9. Jackson, A.L. et al. (2003) Expression profiling reveals off-target gene regulation by RNAi. Nat. Biotechnol. 21, 635.
10. Lewis, B.P., Burge, C.B., and Bartel, D.P. (2005) Conserved seed pairing, often flanked by adenosines, indicates that thousands of human genes are microRNA targets. Cell 120, 15.
11. Lim, L.P. et al. (2005) Microarray analysis shows that some microRNAs downregulate large numbers of target mRNAs. Nature 433, 769.
12. Saxena, S., Jónsson, Z.O., and Dutta, A. (2003) Small RNAs with imperfect match to endogenous mRNA repress translation. Implications for off-target activity of small inhibitory RNA in mammalian cells. J. Biol. Chem. 278, 44312.
13. Judge, A.D., Sood, V., Shaw, J.R., Fang, D., McClintock, K., and MacLachlan, I. (2005) Sequence-dependent stimulation of the mammalian innate immune response by synthetic siRNA. Nat Biotechnol. 23, 457.
14. Hornung, V. et al. (2005) Sequence-specific potent induction of IFN-alpha by short interfering RNA in plasmacytoid dendritic cells through TLR7. Nat Med. 11, 263. 
3' UTR/seed区域分析

研究表明siRNA反义链源区域与非目的靶标mRNA3’非编码区的匹配(见表),可能导致脱靶效应。siRNA双链的反义链上的2-7位是源区域,包括6个碱基。由于siRNA可模拟miRNA的作用,类似的匹配会促进非靶标mRNA的减少。使用QIAGEN设计的siRNA,与源自miRNA,siRNA和鼠RefSeq数据库的3’非编码区专利产品相配合,可对3’UTR/seed区进行分析研究。将每个siRNA与这些序列比对,检查任何可能导致miRNA类脱靶效应的同源序列。

siRNA源区域所有6个碱基与无关靶标3’非编码区序列完全匹配是常见情况,且无需除去这种siRNA。更罕见的是siRNA序列中出现源区域与10个或更多碱基同源匹配的情况,这种同源性很有可能导致脱靶效应,而这些siRNA可能因为与非靶标基因表现出更高的同源性而被弃用。

对于一些靶位点,很难选择到完全非同源性的siRNA。对于这种情况,非相关基因的EntrezGene ID可能是GeneGlobe提供的siRNA的非靶标基因。对这种类型同源性的关注并不意味这些基因一定会受到siRNA的影响,然而如有必要,后续分析中可以认定上述基因为潜在的非靶标基因。

原理

FlexiTube siRNA提供冻干粉形态的siRNA,最小订购规格为1 nmol(最少订购4条siRNA),经济实用,还提供5 nmol和20 nmol的规格。

FlexiTube GeneSolution是针对特定基因的最佳解决方案

只需将详细的人类或小鼠基因信息输入GeneGlobe网站,即可获得适合目标基因的高效RNAi解决方案。搜索结果将显示FlexiTube GeneSolution,每个基因推荐4条1 nmol的siRNA。已发表的文献推荐进行重复性实验,以确保RNAi实验结果(Echeverri, C.J. et al. (2006) Minimizing the risk of reporting false positives in large-scale RNAi screens. Nat. Methods. 3, 777; Echeverri, C.J. and Perrimon, N. (2006) High-throughput RNAi screening in cultured cells: a user’s guide. Nature Reviews Genetics 7, 373)的准确性。在重复性实验中,使用靶定同一mRNA不同区域的不同siRNA来降低脱靶效应。siRNA交叉沉默转录物的具体型可能诱导脱靶表现型。由于该表现型直接来源于siRNA序列,因此不同序列siRNA共享同一序列来源脱靶效应的可能性非常低。使用多个不同siRNA确认一个表现型,以证实siRNA特异性的方法易于使用,且十分可靠。使用FlexiPlate GeneSolution可开展人类和小鼠基因的重复性实验。QIAGEN推荐对每个基因使用siRNA,如此则实验所需的最佳解决方案将触手可及。

提供siRNA的完整序列信息

所有siRNA序列信息在购买siRNA时均免费附赠。完整序列信息可用于实验结果分析和抑制验证。如有需要,siRNA序列信息可用于研究报告中。

修饰选择

FlexiTube siRNA的20 nmol规格可提供标记,包括Alexa Fluor、荧光素、罗丹明、Cy3和Cy5染料,或氨基酸接头、硫代接头和磷酸盐修饰等修饰选择。

程序

对于低通量和高通量siRNA转染,分别推荐使用HiPerFect Transfection Reagent和HiPerFect HTS Reagent。

应用

FlexiTube siRNA和FlexiTube GeneSolution是分析少量靶基因的理想产品,适用于功能基因组学和通路分析。

资源

学术海报 (1)
Poster for download
文章 (1)
Extensively characterized controls for RNAi in human, mouse, and rat
安全数据表 (1)
Download Safety Data Sheets for QIAGEN product components.
基因表达分析 (1)
Safety Data Sheets (1)
Certificates of Analysis (1)

FAQ

How do I calculate the percentage of silencing with real-time RT-PCR for siRNA?

Please find a detailed description for the calculation of the silencing effect in QIAGEN News article 2006 e14 'Real-time RT-PCR for analysis of gene knockdown by RNAi - controls and calculations'.

 

FAQ ID -498
What are the suggestions for unsuccessful gene knockdown?

Determine the transfection efficiency and identify the optimal siRNA concentration for the cell type. Assess the gene knockdown effect at mRNA level using real-time PCR. In some cases, you may need to assess mRNA levels at 48, 72, and 96 hours post-transfection. You may also want to include positive controls for both transfection and gene knockdown experiments.

If the issue persists, send real-time PCR data and/or western blot data to QIAGEN Technical Service for further assistance
FAQ ID -9031
What is the difference between the 1 nmol FlexiTube and FlexiTube Gene Solution siRNAs?

The siRNA sequences are the same.  With FlexiTube siRNA 1 nmol scale, minimum 4 siRNAs required. It can be any human or mouse, any target, 4  different siRNAs, or the same siRNA.   Whereas 1 nmol FlexiTube GeneSolution is a gene-specific package of 4 pre-selected siRNAs for the same target. 

FAQ ID -3174
How long is fluorescence detectable in cells after transfection with fluorescently labeled siRNAs?

Cells transfected with Alexa-Fluor labeled siRNA still show detectable fluorescence 72 hours after transfection. Certain Alexa dyes, e.g. Alexa Fluor 546, are detectable up to one week after transfection. By comparison, when labeling siRNA with Rhodamine or Fluorescein, transfected cells should be monitored for transfection efficiency after 3-4 hours.

Since Alexa Fluor dyes are more photostable, more resistant to variable pH conditions while in transit through the cell, and much brighter than traditionally used fluorescent dyes, Alexa Fluor labeled HPP Grade siRNA is the ideal choice for monitoring transfection efficiency.

For data and additional details on using fluorescently labeled siRNA, refer to QIAGEN News article e20, 2004: 'Alexa Fluor labeled siRNA is highly effective for monitoring transfection efficiency'.

FAQ ID -392
What are the critical factors in designing the siRNA molecules to be used for RNAi studies?
The algorithm utilized to design the siRNA of interest must assure both exquisite gene-specificity (to minimize off-target effects) and potent efficacy (expression knock down). A minimum of two siRNA molecules must be used for each gene of interest, in order to confirm the gene specificity of any observed changes.
FAQ ID -2759
What is the difference between various FlexiTube siRNAs listed for the same target gene, and which one should I choose?

Different Flexitube siRNAs for the same target gene vary slightly in their nucleotide sequence and exact position along the target. All of them were selected by the unique HiPerformance siRNA Design Algorithm and thus have a very high likelihood for knocking down the target gene efficiently. Knockdown achieved with siRNA designed by the HiPerformance algorithm is usually greater than 70%.

Consequently, any of the FlexiTube siRNAs listed in GeneGlobe for a given gene can be chosen for knockdown experiments. We strongly recommend to try at least two siRNAs for independent confirmation that the observed effects are due to specific knockdown of the targeted gene.

Flexitube siRNA comes with a one-time–only replacement offer. If 2 or more HP GenomeWide siRNAs for the same target gene are ordered and none of the siRNAs result in gene silencing, QIAGEN will provide 2 additional siRNAs free of charge, once only. Please visit our website, or contact QIAGEN Technical Services for details and required proof data.

FAQ ID -1206
What are the critical parameters to when optimizing transfection conditions?
The following parameters may be assessed, in an effort to maximize transfection efficiencies:

The amount of siRNA/shRNA being delivered

The optimal amount will be dependent upon the cell line, and target gene, under study. For most experiments, maximal potency, with minimal off-target effects, is achieved between 1nM to 100nM siRNA or shRNA plasmid.

The amount of transfection reagent

This is dependent upon the transfection reagent being used and should be optimized carefully. For QIAGEN’s transfection reagents you will find helpful starting conditions for optimization based on real experimental data on our Transfect Protocol database (http://www.qiagen.com/transfectionprotocols/default.aspx).

Length of transfection complex formation incubation period

Many chemical transfection reagents have a “sweet spot”, at which time a transfection complex of optimal diameter is formed. This is typically between 5 to 30 minutes, depending upon the nature of the reagent. Refer to the reagent manufacturer’s recommendations.

Cell line

Optimal transfection conditions are extremely cell line-dependent. The amount of siRNA/shRNA and transfection reagent, as well as the amount of time that the transfection complex should be left on the cells, will vary from one cell line to another. Helpful information is always available at the Transfect Protocol Database (http://www.qiagen.com/transfectionprotocols/default.aspx).

Cell density

This will be cell line-dependent. For most adherent cell lines, cultures that are 60-80% confluent at the time of transfection are typically optimal. For suspension cultures, densities between 0.5-1.0 X 106 cells/ml are typically optimal.

Cell passage number

Transfection efficiency declines the longer the cells are kept in culture. It is recommended that cell cultures that have been in culture beyond 10 passages NOT be used for transfection. Always take care to make sure that the cell cultures to be transfected are actively dividing, and are at least 90% viable, prior to transfecting.

Traditional vs. reverse transfection protocol

In some instances, plating cells onto wells or plates containing transfection complexes may result in increased transfection efficiency, compared to the traditional approach of adding transfection complexes to an established culture. An additional benefit to such reverse transfection protocols is that seeding and transfecting cells on the same day shortens the experimental timeline by a full day.

Electroporator settings

When utilizing electroporation to deliver siRNA/shRNA to cells that are difficult to transfect via conventional chemical methods, the voltage, pulse length, and pulse number are three critical factors which will require optimization. For additional information, refer to your instrument’s user’s manual.
FAQ ID -9032
Is there a guarantee for the performance of FlexiTube siRNAs in gene knockdown?
Yes. FlexiTube siRNA comes with a one-time–only replacement offer. If 2 or more FlexiTube siRNAs for the same target gene are ordered and two or more do not result in gene silencing, QIAGEN will provide 2 additional siRNAs free of charge, once only. You will be asked to provide supporting data, demonstrating that the siRNA failed to knock down the target gene by at least 70% at the mRNA level under appropriate transfection conditions. Supporting data should include transfection efficiency data, quantitative silencing data, and data showing ≥ 70% knockdown of a positive control. This offer is valid for up to 6 months after the date of delivery.

 

FAQ ID -9040
Do I need to resuspend FlexiTube siRNAs in siRNA Resuspension buffer?

You just need to add sterile RNase-free water (which is supplied with your siRNAs) to resuspend your FlexiTube siRNA. You do not need to perform incubation steps at 96°C or at 37°C. Your siRNA comes preannealed and does not need any further preparation prior to use.

 

FAQ ID -1659
Can I still reorder siRNA that has been removed from the GeneGlobe data base?

Some siRNAs have been deleted from our standard GeneGlobe offering. For those siRNAs, the entries in public databases may have changed and the transcript is no longer listed in those databases. In other cases, we have added siRNAs with a new design.

You can still find previously listed siRNAs in GeneGlobe by searching for the specific SI number (ordering number). See also FAQ 1366 on this topic.

 

FAQ ID -1668
Do I need to anneal, deprotect or desalt my QIAGEN siRNA?

QIAGEN siRNA is delivered as a stable, ready-to-use duplex and does not need to be deprotected, desalted, quantified, or annealed before use. Simply resuspend the lyophilized RNA in the sterile RNAse-free water provided and transfect. Instructions for preparing your siRNA are provided on the data sheet supplied with each siRNA shipment.

FAQ ID -398
What criteria should one use in choosing between siRNA versus shRNA for their studies?

This decision is based on two key factors – the “transfectability” of the target cells, and the desired duration of the experiment.

siRNA molecules work well for high throughput, transient studies, with cells that are easily transfected. The limitations of using siRNA are two-fold. First of all, they do not work well with a few cell types that are extremely difficult to transfect. In addition, their use is restricted to experiments studying the impact of transient suppression of gene expression.

shRNA are carried within the context of a plasmid or viral-based vector, they can be engineered to carry a reporter gene. A reporter gene provides a straightforward readout, for carrying out transfection optimization studies. In addition, a fluorescent reporter gene (such as GFP) allows the use of fluorescence-activated cell sorting (FACS) to enrich for transfected cells. Alternatively, the vector may carry an antibiotic-resistance gene, which permits the selection of a stably transfected cell population. Another obvious advantage to using a vector-based shRNA construct is that it provides a renewable source of reagent for subsequent RNAi studies.

The key benefit of using viral-based shRNA delivery vectors is that they can efficiently deliver the shRNA into cells that are difficult (or impossible) to transfect. Additionally, viral transduction is a much more efficient process than transfection.

FAQ ID -2771
Are Northern Blots sensitive enough to detect siRNA-induced gene silencing?

Yes, Northern Blot Analysis has been shown in the literature to detect siRNA-induced reduction of specific mRNA. Whether a Northern Blot will be sensitive enough to detect a mRNA under investigation mainly depends on the expression level of the respective gene in the untreated control.

You can find an example for this application in the reference "Specific inhibition of gene expression by small double-stranded RNAs in invertebrate and vertebrate systems". Caplen et al., PNAS 2001, vol. 98, no. 17, pages 9742-9747.

We recommend to perform real-time RT-PCR for exact quantification of mRNA expression levels.

FAQ ID -403
Can HP Validated siRNAs be ordered on the FlexiPlate?

Yes, you can order HP GenomeWide siRNAs and HP Validated siRNAs with the Flexiplate siRNA format. There is no price difference between HP GenomeWide siRNAs and HP Validated siRNAs ordered as FlexiPlate siRNA. For HP Validated siRNAs, no sequence information is provided.

 

FAQ ID -1367
Do you have a protocol for the fixation of cells transfected with fluorescently labeled siRNA?

For the fixation of cells transfected with fluorescently labeled siRNA, we would suggest to perform the following protocol:

  1. After transfection, remove the medium from the cells and wash the cells once with PBS.
  2. Incubate the cells for 15 minutes at room temperature with 4% Paraformaldehyde (in PBS, pH 7.0). The cells should be completely covered by this solution (e.g., for a 96-well plate use 50 µl solution/well)
  3. Wash the cells with PBS.

Fixed cells can be stored at 4°C for a few days.

(Note: It is also possible to use chamber slides or object slides for this procedure. Object slides should be coated to provide better growing conditions for cells. Cells can be fixed as described above and then overlayed with embedding medium to allow investigation using a fluorescence microscope. Optimal conditions for this method need to be determined by the user)

 

FAQ ID -793
What controls are important to include in a well designed RNAi experiment?

Negative controls are of critical importance, when performing RNAi studies, in order to confirm that any observed molecular and/or cellular changes are due to the sequence-specific RNAi event. Ideally you should use a scrambled artificial sequence that does not match any of the genes of the cell line/cell type being studied. It is important that appropriate experiments be carried out in advance to validate that the negative control siRNA under consideration has minimal impact on cell viability, proliferation, and global gene expression. The molar amount of negative control siRNA molecules used must be the same as the amount of experimental siRNA that are to be used in the knock down studies.AllStars Negative Control siRNA has been tested thoroughly for potential off target effects and has proven as suitable negative control siRNA already for many years.

Positive controls are also very useful, particularly when carrying out preliminary transfection optimization and/or assay development studies. As with the negative controls, positive controls should be experimentally validated in your model cell line of interest, at the appropriate siRNA concentration, prior to adopting them as acceptable controls. AllStars Cell Death Control siRNA is a phenotypic siRNA, which does not require tedious analysis steps.

 

FAQ ID -9034
What are the critical factors for reliable RNAi validation using qRT-PCR?

 

Our R&D team has carried out an extensive study aimed at answering this question. A thorough evaluation of the major contributing factors essential to RNAi validation using qRT-PCR was carried out. A complete description of this study can be found at the following web address:

 

http://www.sabiosciences.com/manuals/shRNAwhitepaper.pdf

 

The conclusion of this study was that the three most important criteria to meet, in order to establish a reliable RNAi validation protocol, are as follows:

 

• Transfection efficiencies of 80% or higher

 

• Standard deviation in the technical replicate raw Ct values from the qPCR analyses should be no greater than 0.2.

 

• Carry out the experiment with no less than three biological replicates of each target gene-specific siRNA/shRNA and each negative control siRNA/shRNA.

 

FAQ ID -9036
What kind of control should I use in my RNA interference experiments?

"QIAGEN offers a variety of positive and negative control siRNAs. In addition, any of our functionally validated FlexiTube siRNAs are suitable positive controls for RNA interference (RNAi). Our AllStars Negative Control siRNAs, a randomly designed sequence with no known homology to mammalian genes, is the most thoroughly tested and validated negative control siRNA currently available. We strongly recommend to use our RNAi Human/Mouse Starter Kit, which includes HiPerFect Transfection Reagent, Allstars Negative Control siRNA, a positive control siRNA directed against human and mouse MAPK1 (HS/Mm_MAPK1 Control siRNA), and Allstars Hs Cell Death Control siRNA, a phenotypic control siRNA that allows monitoring gene silencing effects by light microscopy." 

FAQ ID -9037
Are FlexiTube siRNA and FlexiTube GeneSolution also available for rat siRNAs?

 FlexiTube siRNA is available for human, mouse and rat genes at 5 nmol and 20 nmol scale. FlexiTube GeneSolution and FlexiTube siRNA at 1 nmol scale are available for human and mouse genes only

FAQ ID -1664
Can FlexiTube siRNA or FlexiTube GeneSolution products be ordered in solution?

No, FlexiTube siRNA and FlexiTube GeneSolution products are only shipped lyophilized at room temperature. We do not offer these products in a different format.

 

 

FAQ ID -1667
What are the structures of the siRNA molecules used in RNAi studies?
The nature of the molecules used in RNAi studies fall into two classes. The first is chemically synthesized siRNA. Typically, these are 21 nt dsRNA molecules with phosphorylated 5’ ends and 3’ dinucleotide overhangs, which directly function as templates for RISC formation. These molecules are introduced via chemical or electroporation-based transfection, and mediate a transient suppression of gene expression. The second class of molecules are shRNA (short hairpin RNA). These are typically delivered to the cell as part of a plasmid or viral vector. The shRNA molecules induce an RNAi effect by serving as substrates for the cytoplasmic RNase, Dicer.
FAQ ID -2760
Can I select HP Validated and HP GenomeWide siRNAs for FlexiTube?

Yes, you can select from HP Validated and HP GenomeWide siRNAs for the FlexiTube format. There is no price difference.

 

FAQ ID -1658
Where can I find QIAGEN products for a specific gene or gene product?
You can search for specific gene products in the QIAGEN GeneGlobe Database. This easy-to-use, comprehensive Web portal allows you to find information about, search for, and order high-quality products for human, mouse, and rat genes. QIAGEN provides a vast range of gene-specific products covering every aspect of an experiment, from gene silencing to expression analysis at the mRNA or protein level.
FAQ ID -803
How do I submit a siRNA order by telephone or online?

FlexiTube siRNA, FlexiTube GeneSolution, FlexiTube siRNA Premix, FlexiPlate siRNA, and GeneFamily Lists siRNAs can be ordered by catalog number over the telephone.

However, to ensure accuracy, Custom siRNA Synthesis orders should be submitted in writing. Therefore you can use the HP Custom siRNA Order Form https://www.qiagen.com/products/genesilencing/customsirna/customsirnaorder.aspx?EmailOrdering=1.

Visit the RNAi Solutions page http://www.qiagen.com/products/rnai/default.aspx?r=2714 on our homepage for access to the Online Ordering Tool, and choose the order link for your product of interest.

FAQ ID -399
If I am working with a difficult-to-transfect cell type or if I obtain only weak silencing effects what can I do?
In the case of difficult cell types or weak silencing effects, it may be helpful to increase the final siRNA concentration during transfection. This can be achieved simply by using larger amounts of FlexiTube siRNA Premix for transfection.
FAQ ID -2265
Do you have information on in vivo RNA interference experiments?

Yes. Please see the QIAGEN News Article (2005 e3) "RNAi - a promising tool for target validation studies and therapeutics" to learn about the most recent advances in this field. It provides numerous references for the aspects of in vivo siRNA delivery and siRNA stability as well as in vivo RNAi in general. QIAGEN offers economical, high-purity siRNA compatible with in vivo animal delivery systems for reliable World-class RNAi solutions.

 

 

FAQ ID -817
Can the MAPK1 control siRNA be used for rat cells?
No. The Mm/Hs_MAPK1 control siRNA is specific for mouse and human MAPK1 only. Please visit GeneGlobe to search for all currently available gene-specific products for RNAi.
FAQ ID -547
Is sequence information for HP Validated siRNAs provided in the FlexiTube format?

Yes, sequence information for FlexiTube is provided both for HP GenomeWide siRNAs and HP Validated siRNAs, in the enclosed paper documentation upon delivery.

 

 

 

FAQ ID -1665
Are your FlexiTube siRNAs preferentially designed to any particular region of the target gene?

No, the design of Flexitube siRNAs in GeneGlobe is not biased towards either the 3' or the 5' end of the target gene.

A number of siRNAs are located in the 3' untranslated region for optimized specificity of the siRNA sequences to their target gene. Since there are homologous sequences in the coding regions of other genes for many targets, it is usually easier to find highly unique siRNA sequences in the untranslated regions. Such design ensures highly specific silencing effects for the gene of interest. 

FAQ ID -1091
What is the most reliable transfection reagent for delivering shRNA plasmids and siRNA to cells in culture?

HiPerFect Transfection Reagent is optimized for siRNA transfections and enables effective siRNA uptake and efficient release of siRNA inside cells, resulting in high gene knockdown even when using low siRNA concentrations. For high-throughput siRNA screenings HiPerFect HTS Reagent is a fast and effective newcomer specifically designed to focus on robustness and cost efficiency. For the transfection of shRNA.

Attractene Transfection Reagent should be used for the transfection of shRNA (short-hairpin RNA) vectors for gene silencing experiments to achieve high efficiency. Ease and flexibility of handling enables preparation and storage of transfection complexes making Attractene Reagent suitable for use with automated systems.

http://www.sabiosciences.com/reversetransfection.php

FAQ ID -2777
Is FlexiTube GeneSolution available for other scales than the 1 nmol scale?
FlexiTube GeneSolution is only available at the 1 nmol scale in tubes.
FAQ ID -1666
What are the most popular methods for monitoring the delivery of a siRNA/shRNA?

Fluorescently-labeled siRNA molecules have been shown to be transfected and processed in a manner that is indistinguishable from unlabeled siRNA. Therefore, these molecules serve as a powerful tool for simultaneously optimizing both siRNA transfection efficiency and the knock down of gene expression. FlexiTube siRNA and HP Custom siRNA is available at 20 nmol scale with different fluorescence labels including AlexaFluor dyes.

Quantitative gene expression analysis via a quantitative reverse transcription-PCR (qRT-PCR) assay is the gold standard for assessing the extent of gene expression knock down in an RNAi experiment. Alternative RNA detection methods, such as Northern blots, RNase protection assays, or end-point PCR, are not quantitative enough to reliably validate gene expression knock down. The RT2 qPCR Primer Assays are available for any gene in the human, mouse, or rat genome. Using these in combination with the pre-optimized RT2 SYBR Green Mastermixes, and the RT2 First Strand Kit provides the easiest, and most reliable, method for quickly evaluating the effectiveness of your gene expression knock down protocol.

Monitoring expression at the protein level via Western blot analysis, ELISA, immunofluorescence, or a functional assay is a critical step in confirming that a gene expression knock down experiment is ultimately resulting in decreased protein levels. However, it is very important to bear in mind that the kinetics of RNA knock down and protein knock down do not usually parallel one another. If the protein under study has a long half-life, then changes in protein level will take much longer to occur than changes in the RNA level. Additionally, it is important to keep in mind that the quality of any antibody-based protein detection assay is dependent upon the quality of the antibody being used.

Phenotypic change in the cells following siRNA delivery, can sometimes be a useful readout for monitoring the effectiveness of an RNAi experiment. AllStars Cell Death Control siRNA is a phenotypic siRNA that has been developed to work in virtually all cell times, as it consists of a blend of siRNAs addressing different vital pathways.

 

FAQ ID -9035
Has RNAi been successful using siRNA in Zebrafish and Xenopus?

Here are examples of references that describe the inhibition of gene expression by siRNA in Xenopus and Zebrafish:

FAQ ID -400
What are the sequences of the FlexiTube siRNAs?

You will receive the sequences of the FlexiTube siRNAs on the data sheet along with your order.

A graphic representation of the position of HP GenomeWide siRNAs along the target sequence is available for numerous genes on our website. It can be accessed via GeneGlobe after pulling up the target gene of interest, clicking on the 'Gene Symbol' link for the species of interest, and then clicking the link under 'Product name' for details on the gene product of interest.



FAQ ID -851
What is the advantage of using a negative (non-silencing) control siRNA labeled with Alexa Fluor 488?

The Alexa Fluor 488 fluorophore is brighter and more photostable than other fluorescent labels. It is tolerant of pH changes within a wide range, making it very stable in living cells. For example, fuorescence microscopy of cells transfected with Alexa Fluor- and FITC-labeled siRNAs after 24 hours showed that the signal of the Alexa Fluor fluorophore was much more persistent than that of FITC. 

FAQ ID -9033
What is the most effective method for validating gene expression knock down in an RNAi experiment?

 

The most accurate method for validating RNA interference is to carry out qRT-PCR on RNA isolated from an enriched or selected population of transfected cells. When carrying out these assays, special care should be taken to insure that highly reproducible biological replicates, as well as technical replicates of the qRT-PCR analysis are performed. This will enable the reliable detection of the roughly 1.75 to 2.0 threshold cycle differences between gene-specific and negative control siRNA/ shRNA transfected cells, which are typically seen in RNAi experiments.

 

QIAGEN has performed intensive validation experiments for FlexiTube and FlexiPlate siRNAs resulting in more than 3700 experimentally tested siRNA now available at GeneGlobe.

 

FAQ ID -9038
What ought I do when working with a difficult to transfect cell type or if I obtain only weak silencing effects?

In the case of difficult cell types or weak silencing effects, it may be helpful to increase the final siRNA concentration during transfection. This can be achieved simply by using larger amounts of FlexiTube siRNA Premix for transfection.

FAQ ID -9039