WIKI資訊
Competitive RT-PCR Strategy for Quantitative Evaluation of the Expression of Tilapia (Oreochromis niloticus) Growth Hormone Receptor Type IQuantization of gene expression requires that an accurate measurement of a specific transcript is made. In this paper, a quantitative reverse transcription-polymerase chain reaction (RT-PCR) by competition for tilapia growth hormone receptor type I is designed and validated. This ......閱讀全文
Competitive RT-PCR in Different Tilapia TissuesAbundance levels of tiGHR I mRNA (target) in different tilapia tissues were measured using the quantita
PCRPolymerase Chain Reaction1) Add the following to a microfuge tube:10 ul reaction buffer1 ul 15 uM forward primer1 ul 15 uM reverse primer1 ul templ
We have also been able to detect expression of this receptor in all studied tissues, which is consistent with the pleiotropic nature of growth hormone
References1. Torre LA, Bray F, Siegel RL, Ferlay J, Lortet-Tieulent J, Jemal A. Global cancer statistics, 2012. CA: a cancer journal for clinician
人胚腎 293 (HEK293) 細胞在重組蛋白表達中是最常見的宿主細胞。 這類細胞能夠表達大量的膜蛋白,如 G 蛋白偶聯受體 (GPCR) ,是無法在最常見的生物制藥生產宿主,如:中國倉鼠卵巢 (CHO) 細胞中作表達。 HEK293 雖然是蛋白表達的極好宿主,然而 H
NGS 是一種識別和確認未知致病菌的前景廣闊的技術,然而其在生物防御和公共健康應用等方面的時效性,卻往往因為缺乏快速、有效、可靠的自動DNA樣品制備方法而受到限制。為了突破這種限制,Kim 等設計了一種基于流體分布元件的數字微流體(DMF) 平臺,使得多子系統模塊能夠進入自動NGS庫樣品
Figure 5: Regulation of CDH5 by TFZFs in several human cancer cell lines.Blue, cells infected with a pMX construct containing the DNA bindin
作者:柳建磊,秦進 作者單位:(成都鐵路中心醫院,四川 成都 610081)【摘要】 目的:建立一種利用MGB-Taqman探針的快速、靈敏、特異、準確定量檢測外周血PSMA mRNA的方法。方法:選擇PSMA mRNA的保守區域,設計合成引
FL3500雙調制葉綠素熒光儀 (新升級型號為FL6000) FL3500雙調制葉綠素熒光儀是專門用于對藍綠藻或綠藻等微藻,葉綠體或類囊體懸浮物,乃至葉片進行光合作用研究的強大科研工具。儀器具備雙通道測量控制,可控制測量樣品的溫度,并配備單翻轉光(STF),內置多種可用戶自行修改的測量程序
第五屆金屬組學國際研討會會議日程 Scientific Programme Wednesday, 9th Sept 2015 9:00 -21:00 Registration Wednesday, 9th Sept 2015, Ginkgo Hall
9月3日,頂級學術期刊《自然》(Nature)發布蘭州大學110周年校慶專刊,以“The buzz from China’s west”為題介紹蘭州大學的歷史及發展,以“Blazing a trail”為題發布了對蘭州大學校長嚴純華的專訪,還分別介紹了蘭州大學生命科學、大氣科學、醫學、草業科學、
生物分子發表的代表性文獻 QTRAP:同時具有三重四極桿和線性離子阱性能的獨一無二的LC/MS/MS系統 QTRAP系統最早在ASMS 2002上,作為第一臺商用的線性離子阱發布,是世界上唯一的線性離子阱和三重四極桿的復合
Table 2: Binding sites and identity of ZFPs used in VEGF activationWe then generated artificial transcription factors by fusing the three-fi
Figure 2: Verification of C1 Single-Cell mRNA-Seq data quality. a)ERCC RNA Spike-In Control Mix 1 was applied to a C1 IFC at a total &nbs
I. INTRODUCTION 引言 This guidance helps sponsors of investigational new drug applications (INDs) or applicants of new drug applications (NDAs),
Determination of Accuracy of the Competitive PCRTo test the precision of the results obtained with this competitive PCR, five different amounts of T (
加拿大Alberta大學 Li, Liang(厲良)教授 來自加拿大Alberta大學的Li, Liang(厲良)教授,做了題為:“Development of LC/MS Techniques fo
實驗概要The SuperScript? III One-Step RT-PCR System with Platinum? Taq High Fidelity is designed for sensitive, high-fidelity end-p
The RT-PCR method can be used not only to detect specific mRNAs but also to semi-quantitate their levels. Thus, one can compare levels of transcripts
Scanning the human genome with combinatorial transcription factor librariesPublished online: 18 February 2003, doi:10.1038/nbt794March 2003 Volume 21
主要內容如下:· RT-PCR· Competitive and Quantative
SummaryQuantitative PCR is a method used to detect relative or absolute gene expression level. All qPCR involves the use of fluorescence to detect the
Application: Quantitative RT-PCR is used to quantify mRNA in both relative and absolute terms. It can be applied for the quantification of m
Protocols for LCM preparation and analysis I. Preparation, LCM and RNA/DNA extraction of Frozen Tissue SectionsA. EmbeddingB. CuttingC.
芯片毛細管電泳具有進樣量少,靈敏度高,分析速度快等特點,非常適合法醫DNA-STR的快速檢驗。毛細管電泳芯片由于尺寸小,可施加較大場強,所以在幾秒鐘內就可完成對樣品的分離,微陣列毛細管電泳芯片可實現高通量檢測則成為目前學者研究的熱點。2002年Emrich CA等[31]報道的將高通量384孔毛
蛋白質組數據處理暨第三屆全國生物質譜學術交流會(第三輪通知) 為了積極促進我國蛋白質組學技術發展和應用、數據挖掘和生物質譜的經驗交流,由中國生物化學與分子生物學會蛋白質組學專業委員會、中國質譜學會生物質譜專業委員會和中國化學會分析化學委員會主辦,北京蛋白質組研究中心、復旦大學和蛋
瑞士蘇黎世聯邦理工學院的研究人員領導的一個研究小組,已制定了一個質譜工作流,用于對整個蛋白質組進行高通量的絕對定量。 據ETH的研究者、該研究的領頭人Ruedi Aebersold說,對于多種形態,該技術實現了目標蛋白質組的重現性定量,提供用于
FluidFM 測定細胞粘附力的應用隨著時間推移,越來越多的學者開始使用FluidFM 技術進行測定細胞粘附力。以下就近五年的具有代表性的應用進行總結。Cohen 等使用FluidFM 技術對MCF7-MCF10A、MCF7-HS5 的細胞粘附力進行了測定,并與以往的文獻進行對比,發現其數據與Hos
In the polymerase chain reaction (PCR), a thermostable DNA polymerase amplifies DNA that is flanked by known sequences. The known sequences correspond
即將向全球推廣的狂犬病實驗診斷新方法----實時定量RT-PCR檢測法(簡稱LN34檢測法),可能作為狂犬病基本檢測診斷方法,補充或取代當前的金標準:DFA檢測。動物和人狂犬病的確診,必須要有實驗室檢測結果,否則都只能算疑似病例。目前WHO(世界衛生組織)肯定的人和動物狂犬病的死后診斷的金標準,是直