Clariom™ S Assay,人类
Clariom™ S Assay,人类
Applied Biosystems™

Clariom™ S Assay,人类

对人类样品采用 Clariom S Assay,以获得基因水平的人类转录组视图。Clariom S 分析作为下一代全转录组基因水平表达谱分析工具,为您的研究提供较快速、简单、可扩展的所需结果生成途径。新型了解更多信息
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货号阵列数量
90292730 阵列
货号 902927
价格(CNY)
-
阵列数量:
30 阵列
对人类样品采用 Clariom S Assay,以获得基因水平的人类转录组视图。Clariom S 分析作为下一代全转录组基因水平表达谱分析工具,为您的研究提供较快速、简单、可扩展的所需结果生成途径。新型 Human Clariom S Assay 基于业内领先的微阵列技术,可广泛涵盖所有已知的带注释基因,并与研究样品类型、可扩展格式和灵活的数据分析软件兼容。Clariom S Assay 是一种尽可能快速、简单、经济地找到具有已知功能的表达生物标记物的工具。

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虽然近年来已知转录基因数量迅速扩大,但对每个基因的功能了解仍在不断加深。数据库中发现的许多基因和转录本的注释不正确或未注释,可能会使数据分析和解释复杂化并延长其时间。Human Clariom S Assay 集中于注释良好的基因,可为研究人员提供展开基因水平表达谱分析研究的能力,并快速评估关键基因和信号通路的变化。Clariom S 人测定试剂盒所需的数据分析时间较短,可帮助研究人员更快地得出结论。

简单、快速发现生物标记物
•准确测量 > 20,000 个良好注释基因的基因水平表达,从而快速得出结果。• 选择一种符合通量需求的规格,处理量范围为每日1至192份样品。•采用专为生物学家设计的直观、高度可视化、免费分析软件,在数分钟内即可从数据获得结果

当有珍贵样品时,一次获得正确结果
• 从总 RNA 量低至 100 pg 的样品中–低至 10 个细胞样品,生成具有可靠性的表达谱。
• 使用来自不同样品类型的 RNA,包括血液、细胞、新鲜/新鲜冷冻或 FFPE 组织。
•通过无需去除球蛋白或 rRNA 步骤的测定,保持样品完整性并降低数据差异性。
•采用全自动样品制备选项,可节省时间和成本。

Clariom S 解决方案可用于在 GeneChip ™ 3000 仪器系统上进行单样品(检测盒阵列)处理和 GeneTitan ™ 微阵列系统上进行高通量自动处理(板阵列),从而提供适合小型和大型队列研究的灵活性。完整溶液包含试剂和快速简单的转录组分析控制台 (TAC) 软件,可在数分钟内分析和显示基因、通路和网络相互作用的整体表达模式。

获取更真实的基因表达水平
为了进行更稳健的基因水平表达谱分析,Human Clariom S Assay 仅检测存在于所有已知转录本亚型中的外显子,这些外显子由单个基因位点所组成的外显子表达。这与其他基因水平的阵列技术和浅层 RNA 测序不同,后者提供了对基因表达的偏倚或因转录本变体表达变化而复杂的数据。Human Clariom S Assay 只能测定每个已知基因长度的组成型外显子,从而生成目前更准确、真实的基因表达测量结果。

Human Clariom S Assay 可简单快速鉴定整个转录组中的生物标记物,使您获得所需要的覆盖范围、所需的可重现性以及有意在发现中发挥作用的结果。
仅供科研使用。不可用于诊断程序。
规格
产品线Applied Biosystems™
数量30 次反应
运输条件经批准可在室温下或者湿冰或干冰上运输
类型S 检测
数组转录组谱分析
产品规格阵列检测盒
阵列数量30 阵列
种属
Unit SizeEach

常见问题解答 (FAQ)

What reagent kit should I use with my array?

Please refer to the Microarray Reagent Guide for Arrays and Expression Kits to match the correct reagents your array.

Find additional tips, troubleshooting help, and resources within our Microarray Analysis Support Center.

Why is it important to use Tough-Spots® labels when using GeneChip cartridge arrays?

Tough-Spots® labels are small adhesive stickers used to temporarily seal the backs of cartridge arrays during the overnight hybridization step. They are required to prevent loss of volume due to evaporation through the septa. We recommend using Tough-Spots® labels on Rolls from USA Scientific (Item No. 9185-0000)

Find additional tips, troubleshooting help, and resources within our Microarray Analysis Support Center.

What are the respective hybridization volumes based on array format for Affymetrix gene expression arrays?

Proper hybridization volume is critical to obtaining an even signal across a given array. Too little volume can lead to black circles in the middle of the array. Too much volume can leak out of the back of the array. The correct hybridization volume leaves enough room for a small air bubble to circulate around the array surface during the overnight hybridization. Here are the recommended hybridization and fill volumes based on the array format:
Array Format; Hybridization Volume; Fill Volume
- 49 Format (Standard); 200 µL; 250 µL
- 64 Format; 200 µL; 250 µL
- 100 Format (Midi); 130 µL; 160 µL
- 169 Format (Mini); 80 µL; 100 µL
- 400 Format (Micro); 80 µL; 100µL

Find additional tips, troubleshooting help, and resources within our Microarray Analysis Support Center.

Why is strand-specificity important when performing Clariom D and Clariom S assays?

Clariom D arrays have probes that cover all known regions of transcription including probes in overlapping regions from both strands. To obtain strand-specific information from the Clariom D arrays, the WT Pico and WT Plus reagents (which are strand-specific) must be used. This is important because without strand-specific reagent, it would not be possible to decipher the source strand of DNA, which makes it challenging to untangle true gene- and exon- level expression and alternative splicing events.

Strand-specificity is significantly less important for customers interested in gene-level only information (i.e., those using Clariom S) as compared to customers who want to understand the complexities of the whole transcriptome including identifying antisense transcripts and ncRNA (i.e., those using Clariom D). While strand-specificity is less important for gene-level expression only, probes within regions of overlapping transcription from both strands are avoided in the Clariom S array design (unlike Clariom D). This is important because if Clariom S did not preserve strand-specificity, there could be an overestimation of gene-level expression causing false positive or negative results. With Clariom S having a "stranded" design, it does not necessarily need a strand-specific reagent kit.

Find additional tips, troubleshooting help, and resources within our Microarray Analysis Support Center.

What is an Event Score in TAC 4.0 Software?

TAC 4.0 includes two algorithms for identifying alternative splicing events: the TAC 2.0 algorithm and the new EventPointer. Algorithmic determination of alternate splicing remains a challenging problem. TAC 4.0 supports two different approaches that have different sets of strengths and weaknesses. After considerable testing, the new TAC 4.0 “'Event Score” leverages both previous TAC 2.0 event estimation score and Event Pointer p-value and sorts the most likely alternative splicing events to the top. Of course, the TAC 2.0 event score and EventPointer p-values remain individually available.

Find additional tips, troubleshooting help, and resources within our Microarray Analysis Support Center.

View all Clariom™ S Assay,人类 FAQs