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IF>5000經(jīng)典預(yù)混液Hieff^? qPCR SYBR Green Master Mix(No Rox)

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產(chǎn)品描述

Hieff® qPCR SYBR Green Master Mix(No Rox)是2×實(shí)時定量PCR擴(kuò)增的預(yù)混合溶液。Mix中含有熱啟動Hieff^® DNA Polymerase、SYBR Green I、dNTPs、Mg²⁺。使用時，僅需在擴(kuò)增體系中加入模板和引物即可進(jìn)行實(shí)時熒光定量PCR，大大簡化操作過程，降低污染幾率。

本品采用的DNA聚合酶配體可以隨溫度變化實(shí)時調(diào)節(jié)DNA聚合酶活性。配方添加了有效抑制非特異性PCR擴(kuò)增的因子和提升PCR反應(yīng)擴(kuò)增效率的因子，使定量PCR可以在寬廣的定量區(qū)域內(nèi)獲得良好的線性關(guān)系。

適用機(jī)型

Bio-Rad: CFX96, CFX384, iCycler iQ, iQ5, MyiQ, MiniOpticon, Opticon,Opticon 2, Chromo4;

Eppendorf: Mastercycler ep realplex, realplex 2 s;

Qiagen: Corbett Rotor-Gene Q, Rotor-Gene 3000, Rotor-Gene 6000;

Roche Applied Science: LightCycler 480, LightCycler 2.0; Lightcycler96;

Thermo Scientific: PikoReal Cycler; Cepheid: SmartCycler; Illumina: Eco qPCR.

運(yùn)輸和保存方式

冰袋運(yùn)輸。-20℃避光儲存，有效期18個月。

本品避免反復(fù)凍融。產(chǎn)品中含有熒光染料SYBR Green I，保存或配制反應(yīng)體系時需避免強(qiáng)光照射。

注意事項(xiàng)

1. 推薦使用本公司cDNA合成試劑盒（貨號：11123ES），以有效去除RNA樣品中殘留的基因組。

2. 解凍后Master Mix可能出現(xiàn)絮狀物質(zhì)，4℃放置并上下顛倒混勻至溶液澄清，不影響試劑性能。

3. 為了您的安全和健康，請穿實(shí)驗(yàn)服并佩戴一次性手套操作。

4. 本產(chǎn)品僅作科研用途！

反應(yīng)體系（推薦冰上配制）

組分	體積（μL）	體積（μL）	終濃度
Hieff® qPCR SYBR Green Master Mix (No Rox)	25	10	1×
Forward Primer (10 μM)	1	0.4	0.2 μM
Reverse Primer (10 μM)	1	0.4	0.2 μM
模板DNA	X	X	-
無菌超純水	to 50	to 20	-

【注】：使用前務(wù)必充分混勻，避免劇烈震蕩產(chǎn)生過多氣泡。

a) 引物濃度：通常引物終濃度為0.2 μM，也可以根據(jù)情況在0.1-1.0 μM之間進(jìn)行調(diào)整。

b) 模板濃度：如模板類型為未稀釋cDNA原液，使用體積不應(yīng)超過qPCR反應(yīng)總體積的1/10。

c) 模板稀釋：cDNA原液建議5-10倍稀釋，最佳模板加入量以擴(kuò)增得到的CT值在20-30個循環(huán)為好。

d) 反應(yīng)體系：推薦使用20 μL或50 μL，以保證目的基因擴(kuò)增的有效性和重復(fù)性。

e) 體系配制：請于超凈工作臺內(nèi)配制，并使用無核酸酶殘留的槍頭、反應(yīng)管；推薦使用帶濾芯的槍頭。避免交叉污染和氣溶膠污染。

【注】: 高特異性可選擇兩步法，高效率擴(kuò)增可選擇三步法。

a) 預(yù)變性時間：根據(jù)不同模板和引物的具體情況可適當(dāng)縮短至2 min。

b) 退火溫度和時間：請根據(jù)引物和目的基因的長度進(jìn)行調(diào)整。

c) 熒光信號采集（^★）：請按照儀器使用說明書要求進(jìn)行實(shí)驗(yàn)程序設(shè)置，幾種常見儀器的時間設(shè)定如下：

30sec以上：Applied Biosystems: StepOne, StepOne Plus, 7500 Fast；Roche Applied Science: LightCycler 480；Bio-Rad: CFX96

31sec以上：Applied Biosystems: 7300

34sec以上：Applied Biosystems: 7500

d) 熔解曲線：通常情況下可以使用儀器默認(rèn)程序。

結(jié)果分析

定量實(shí)驗(yàn)至少需要三個生物學(xué)重復(fù)。反應(yīng)結(jié)束后需要確認(rèn)擴(kuò)增曲線及熔解曲線。

1) 擴(kuò)增曲線：標(biāo)準(zhǔn)擴(kuò)增曲線為S型。

Ct值落在20-30之間時，定量分析最準(zhǔn)確；

Ct值小于10時，需要將稀釋模板后，重新進(jìn)行實(shí)驗(yàn)；

Ct值介于30-35之間時，需要提高模板濃度，或者增大反應(yīng)體系的體積，以提高擴(kuò)增效率，保證結(jié)果分析的準(zhǔn)確性；

Ct值大于35時，檢測結(jié)果無法定量分析基因的表達(dá)量，但可用于定性分析。

2) 熔解曲線：

熔解曲線單峰，表明反應(yīng)特異性好可以進(jìn)行定量結(jié)果分析；若熔解曲線出現(xiàn)雙峰或者多峰，則不能進(jìn)行定量分析。

熔解曲線出現(xiàn)雙峰，需要通過DNA瓊脂糖凝膠電泳判斷非目標(biāo)峰是引物二聚體還是非特異性擴(kuò)增。

如果是引物二聚體，建議降低引物濃度，或者重新設(shè)計(jì)擴(kuò)增效率高的引物。

如果是非特異性擴(kuò)增，請?zhí)岣咄嘶饻囟?，或者重新設(shè)計(jì)更高特異性的引物。

引物設(shè)計(jì)指南

1. 推薦引物長度25 bp左右。擴(kuò)增產(chǎn)物長度150 bp為佳，可以在100 bp-300 bp內(nèi)選擇。

2. 正向引物和反向引物的Tm值相差不宜超過2℃。引物Tm值60℃-65℃為佳。

3. 引物堿基分布要均勻，避免出現(xiàn)連續(xù)的4個相同堿基，GC含量控制在50%左右。3’端最后一個堿基最好為G或C。

4. 引物內(nèi)部或者正反兩條引物間最好避免出現(xiàn)有3個堿基以上的互補(bǔ)序列。

5. 引物特異性需要用NCBI BLAST程序進(jìn)行核對。避免引物3’端有2個堿基以上的非特異性互補(bǔ)。

6. 設(shè)計(jì)完成的引物需要進(jìn)行擴(kuò)增效率的檢測，只有具備相同擴(kuò)增效率的引物才可用于定量比較分析。

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Hifair^® II 1st Strand cDNA Synthesis Kit ^HOT	11119ES60	100 T
Hifair ^® II 1st Strand cDNA Synthesis Kit (gDNA digester plus)	11121ES60	100 T
Hifair ^® II 1st Strand cDNA Synthesis SuperMix for qPCR(gDNA digester plus)^HOT	11123ES60	100 T
Hieff ^® qPCR SYBR® Green Master Mix (No Rox )^HOT	11201ES08	5 ml
Hieff ^® qPCR SYBR® Green Master Mix (Low Rox Plus) ^HOT	11202ES08	5 ml
Hieff ^® qPCR SYBR® Green Master Mix (High Rox Plus) ^HOT	11203ES08	5 ml

HB210720

Q：不加 ROX 的qPCR mix 后續(xù)需換用其他儀器（需要 ROX），是否可以單獨(dú)加 ROX后再使用？

A：可以。

Q：可以用于microRNA 或lncRNA 等非編碼RNA 嗎？環(huán)狀 RNA 呢？

A：不推薦。

Q：建議qPCR 實(shí)驗(yàn)用幾步法？

A：常用 2 步法。需提高擴(kuò)增特異性，可選用 2 步法或提高退火溫度。在擴(kuò)增效率低， ct 值過大的時候，可以改用 3 步法或延長延伸時間。

Q：預(yù)變性 5 min 調(diào)整成了 10min，對于實(shí)驗(yàn)結(jié)果有影響嗎？

A：有影響，預(yù)變性時間較長可能會影響酶的活性，導(dǎo)致 PCR 產(chǎn)物的產(chǎn)量有所降低。

Q：qPCR 實(shí)驗(yàn)結(jié)果的有效性？為什么建議Ct 值要大于 15？

A：有效性要滿足三個條件：（1）標(biāo)準(zhǔn)曲線：擴(kuò)增效率范圍:90-110%，對應(yīng)斜率為 -3--3.5。 R2＞0.98。 (擴(kuò)增效率=10-1/斜率-1)，當(dāng)斜率=-3.32 時，擴(kuò)增效率=100%。（2）擴(kuò) 增曲線：S 型曲線，且 Ct 值在 15－35 之間，陰性對照 Ct＞35 或無 Ct 值。（3）熔解曲線：為單一峰。

Ct 值大于 15 個循環(huán)是因?yàn)?/font> 3-15 個循環(huán)的熒光值標(biāo)準(zhǔn)差的 10 倍是熒光閾值，Ct 值太小了會影響曲線。

Q：同一基因復(fù)孔間熔解曲線 Tm 值有差異？

A：同樣的擴(kuò)增產(chǎn)物也會出現(xiàn)Tm 值有微小差異，一般差異在 1 度以內(nèi)都可以接受。

Q：為什么稀釋了模板CT 值反而變小了？

A：一般 CT 值與模板起始濃度呈負(fù)相關(guān)，濃度越高，CT 值越小。但也有很多特殊情況，比如體系中存在抑制物或是模板不純，這時候稀釋模板反而能使 CT 值變低。

Q：11201,11202,11203區(qū)別是什么呢？如何選擇呢？

A：里面預(yù)混的ROX濃度不同，需要根據(jù)儀器的型號進(jìn)行對應(yīng)選擇。

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