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Molecular Cloning Laboratories(MCLAB)成立于1998年,是为生命科学界提供基因组研究耗材和服务的先进者。

MCLAB提供具有成本效益的消耗品和试剂,专注于代以及新一代测序和DNA段分析。我们提供大量分子生物学相关产品,包括抗体,生化试剂,克隆试剂盒,酶,PCR试剂盒,蛋白质凝胶和溶液等。作为我们自己的制造商,我们可以控制生产流程,并大限度地减少定制和大规模订单的延迟。它有助于确保我们的客户获得高质量和价值。

MCLAB拥有一支由20 多位经验丰富的科学家组成的团队,致力于为研究人员提供的服务。我们专注于基因组学领域,拥有DNA测序,发酵,片段分析,分子克隆,过表达,蛋白质纯化和蛋白质合成方面的专家。我们采用量身定制的客户服务方式,让您有机会定制您的项目,并直接与我们的科学家团队交流以获得技术支持。凭借二十多年的经验,我们才华横溢,技术的员工致力于为您提供所需的成果。

RT-PCR试剂盒

链cDNA合成试剂盒

First Strand cDNA Synthesis Kit

链cDNA合成试剂盒可用于合成链cDNA。

名称

货号

描述

链cDNA合成试剂盒

FSCS-100

50次反应

链cDNA合成试剂盒

FSCS-200

250次反应

 

 

 

 

描述:
链cDNA合成试剂盒可用于在比野生型M-MuLV更高的温度下通过逆转录(RT)合成链cDNA,并且基于MCLAB的QuantumScript™可以获得更高的cDNA转录率以进行困难的RNA转录HD逆转录酶,一种独特的突变,可提高热稳定性并降低RNase H活性。

应用:
- cDNA合成
- RT-PCR 
- RT-qPCR

储存条件:
-20°C。建议尽可能少地减少冻融循环。

 

 

 

 

部分产品:

名称

货号

尺寸

浓度

大肠杆菌DNA连接酶

EDLA-100

1,000个单位

10,000 U / ml

大肠杆菌DNA连接酶

EDLA-200

5,000个单位

10,000 U / ml

大肠杆菌DNA连接酶

EDLA-OEM

任何尺寸

 

 

APE 1

APE-100

3,750 units

15,000 U/ml

APE 1

APE-200

15,000 units

15,000 U/ml

APE 1

APE-OEM

Any Size

 

 

名称

货号

描述

I-5™2X高保真混色

I5HM-100

100次反应(50μl体积)

I-5™2X高保真混色

I5HM-200

500次反应(50μl体积)

I-5™2X高保真混色

I5HM-5000

5,000次反应(50μl体积)

I-5™2X高保真混色

I5HM-25K

25,000次反应(50μl体积)

I-5™2X高保真混色

I5HM-OEM

OEM

名称

货号

描述

2x BlueStar™PCR Master Mix

BSPM-100

100次反应(50μl体积)

2x BlueStar™PCR Master Mix

BSPM-200

1,000次反应(50μl体积)

 

名称

货号

尺寸

HoTaq DNA聚合酶(热启动)

HT-200

500个单位,5 U /μl

HoTaq DNA聚合酶(热启动)

HT-205

2,500个单位,5 U /μl

HoTaq DNA聚合酶(热启动)

HT-210

5,000单位,5 U /μl

HoTaq DNA聚合酶(热启动)

HT-OEM

任何尺寸

名称

货号

描述

10 x PBS(磷酸盐缓冲盐水)

PBS10-100

500毫升

10 x PBS(磷酸盐缓冲盐水)

PBS10-200

1升

10 x PBS(磷酸盐缓冲盐水)

PBS10-OEM

OEM

 

 

 

 

 

 

 

名称

货号

描述

I-5™Hi-Fi DNA聚合酶

PDP-100

250单位,2.5 U /μl

I-5™Hi-Fi DNA聚合酶

PDP-200

1,250单位,2.5 U /μl

I-5™Hi-Fi DNA聚合酶

PDP-OEM

任何尺寸

 

名称

货号

描述

I-5™Hotstart DNA聚合酶

I5HD-100

250单位,2.5 U /μl

I-5™Hotstart DNA聚合酶

I5HD-200

1,250单位,2.5 U /μl

I-5™Hotstart DNA聚合酶

I5HD-OEM

任何尺寸

名称

货号

尺寸

浓度

Pfu DNA聚合酶

AD-200

500个单位

2.5 U /μl

Pfu DNA聚合酶

AD-205

1,000个单位

2.5 U /μl

Pfu DNA聚合酶

AD-210

2,500个单位

2.5 U /μl

Pfu DNA聚合酶

AD-OEM

任何尺寸

 

 

名称

货号

尺寸

浓度

Taq DNA聚合酶(常规)

TR-100

1,250个单位

5 U /μl

Taq DNA聚合酶(常规)

TR-200

5,000单位

5 U /μl

Taq DNA聚合酶(常规)

TR-OEM

任何尺寸

 

 

名称

货号

描述

All-In-One 5X Reverse Transcription Mix Kit

IO-100

25 rxn(4ul / rxn),100μl

All-In-One 5X Reverse Transcription Mix Kit

IO-200

100 rxn(4ul / rxn),400μl

 

 

上海起发实验试剂有限公司是实验试剂一站式采购服务商

1:强大的进口辐射能力,血清、抗体、耗材、大部分限制进口品等。

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3:提供加急服务,货品一般1-2周到货。

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6:我们还是Santa,Advanced Biotechnologies Inc,Athens Research & Technology,bangs,BBInternational,crystalchem,dianova,FD Neurotechnologies,Inc. FormuMax Scientific,Inc, Genebridege, Glycotope Biotechnology GmbH; iduron,Innovative Research of America, Ludger, neuroprobe,omicronbio, Polysciences,prospecbi, QA-BIO,quickzyme,RESEARCH DIETS,INC,sterlitech;sysy,TriLink BioTechnologies,Inc;worthington-biochem,zyagen等几十家国外公司授权代理。

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Molecular Cloning Laboratories Mclab Nimagen B.v.

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Molecular Cloning Laboratories Mclab Nimagen B.V. Is An Other Supplier(). The Following Data Of Trade Reports Comes From Customs Data. This Company's Import Data Update To 2015-09-11, A Total Of 1 Transactions. Based On These Data, We Made Statistics And Summary From The Trade Partners, Import-Export Ports, Purchasing Countries, HS Codes, And Contact Information. It Will Help You To Improve The Use Sufficiency Of Trade Data. This Picture Is The Market Trend Analysis Of Molecular Cloning Laboratories Mclab Nimagen B.V. About A Near Year And We Can Learn This Company's Procurement Cycle And Business Stability From The Quantity, Weight, Price, And The Number Of Transactions.

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Molecular Cloning Laboratories Mclab Nimagen B.V. Is A Other Supplier, The Data Is From Other Customs Data. This Company's Trade Report Mainly Contains Market Analysis, Contact, Trade Partners, Ports Statistics, And Trade Area Analysis. Official Reference Contact Is From Other Original Bill Of Ladings, Including Email, Phone, Fax, Address, And Official Website. Till 2015-09-11,Molecular Cloning Laboratories Mclab Nimagen B.V. A Total Of 1 Transactions. Follow Up The Company, And Then Can Export This Company's Contact And B/Ls. If There Is New Transactions, We Will Also Inform You By The System.
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Molecular cloning and function analysis of PsMYB18 in 'Akihime' plum (Prunus salicina Lindl.)

FANG Zhizhen;JIANG Cuicui;ZHOU Danrong;PAN Shaolin;LIN Yanjuan;YE Xinfu;Fruit Research Institute,Fujian Academy of Agricultural Sciences/Fujian Engineering and Technology Research Center for Deciduous Fruit Trees,Fujian Academy of Agricultural Sciences;  
【Objective】Temperature and light are important environmental factors that affect the biosynthesis and accumulation of anthocyanin in the fruit peel. Our previous study indicated that 20 ℃ temperature and light treatment(150 mol·m~(-2)·s~(-1)) could induce anthocyanin accumulation in the peel of postharvest'Akihime'plums. Comparative transcriptomic analysis results demonstrated that the expression of a R2 R3-MYB gene(designated as PsMYB18) was significantly upregulated in the fruit peel treated at20 ℃+ light. The objective of the study was to isolate and elucidate the function of PsMYB18 gene during anthocyanin accumulation in the peel of'Akihime'plum.【Methods】The total RNA of the plum fruit peels was extracted using EZNA Plant RNA Kit(Omega Bio-tek, USA) according to manufacturer's instructions. Real-time quantitative PCR(qRT-PCR) was employed to determine the expression of PsMYB18 in the peel of'Akihime'plum fruits treated at 20 ℃ + light, 20 ℃+ dark, 30 ℃+ light and30 ℃+ dark. First-strand cDNA was synthesized from 500 ng of total RNA using the PrimeScript RT reagent kit with gDNA Eraser(Takara, China). The qRT-PCR was performed using the Eppendorf Realplex4 real-time PCR system(Hamburg, Germany) in a total volume of 20 μL in each well containing 10μL of 2×SYBR~? Premix Ex Taq? II(Tli RNaseH Plus, TaKaRa), 1 μL of cDNA(in 1:10 dilution), and0.4 μL 10 μmol primers. The qPCR conditions were 30 s at 95 ℃, followed by 40 cycles of 5 s at 95 ℃,15 s at 60 ℃, and 30 s at 72 ℃, followed by 60 ℃ to 95 ℃ melting curve detection. Actin gene was used as the reference. For gene cloning, total RNA was extracted from the fruit peel treated with 20 ℃and light. The first-strand cDNA was synthesized using First Strand cDNA Synthesis Kit(Thermo Scientific, USA). PsMYB18 gene was isolated from the skin of'Akihime'plums by reverse transcription polymerase chain reaction(RT-PCR). Phylogenetic tree was constructed using the MEGA 5.02 software to investigate the evolution relationship between PsMYB18 and MYB proteins from other plant species.Multiple sequence alignments of PsMYB18 protein with MYB repressors from peach, apple, grape, poplar, Medicago truncatula, Fragaria × ananassa and Antirrhinum majus were performed using DNAMAN7.02. p CAMBIA1302 vector, which was linearized by restriction enzyme NcoI and BstEII was used to construct overexpression vectors. The coding regions of PsMYB18, PsMYB10.1 and PsbHLH3 were isolated using I-5? 2×High-Fidelity Master Mix(MCLAB, San Francisco, CA) and then cloned into the pCAMBIA1302 vector using One Step Seamless Cloning kit(Aidlab, China). All constructs were introduced into Agrobacterium tumefaciens GV3101. Tobacco(Nicotiana tabacum L.) leaf transient expression assay was performed to verify the function of PsMYB18 in anthocyanin biosynthesis. The Agrobacterium strain GV3101 containing overexpression vectors were grown at 28 ℃ in LB medium containing with antibiotics. Then Agrobacterium cells were harvested and resuspended in the infiltration buffer(10 mmol·L~(-1) MgCl2, 10 mmol·L~(-1) MES, pH 5.6, 100 μmol·L~(-1) acetosyringone) to a final OD600 of 0.8. The bacteria were incubated at room temperature for 3 h before infiltration. Digital photographs of anthocyanin development in tobacco leaves were taken at 7 days after infiltration.【Results】The qRTPCR analysis revealed that the expression of PsMYB18 in the fruit peel treated at 20 ℃ and light was significantly enhanced after 3 d of treatment and remained at a high level thereafter. However, no obvious expression upregulation of PsMYB18 was detected in the fruit peel treated at 20 ℃ + dark, 30 ℃ +light and 30 ℃ + dark. These results were consistent with RNA-seq data. The cDNA sequence of PsMYB18 was isolated from the peel of'Akihime'fruits treated at 20 ℃ and light. PsMYB18 contained open reading frame(ORF) of 702 bp in length, which was predicted to encode a protein of 539 amino acid residues. The results of phylogenetic analysis revealed that PsMYB18 and repressors of anthocyanin and proanthocyanidin biosynthesis, including FaMYB1, MtMYB2, PtMYB182, VvMYBC2-L3, VvMYBC2-L1 and PpMYB18, from other plants belonging to the same class. It had the closest relationship with PpMYB18 from peach. Multiple alignment of the deduced amino acid sequences of PsMYB18 and MYB repressors showed that PsMYB18 shared similarity of 96.57% with the PpMYB18 protein and contained the conserved R2 and R3 domains. It also had C1 and C2 repression motifs in the C-terminus. These results implicated that PsMYB18 could be a repressor of anthocyanin biosynthesis.To investigate the role of PsMYB18 in anthocyanin biosynthesis, the ORF of PsMYB18 was amplified and ligated into the pCAMBIA1302 vector. Transient color assays in tobacco leaves showed that coinfiltration of PsMYB18 with PsbHLH3 could not induce anthocyanin accumulation. Furthermore, coinfiltration of PsMYB10.1 with PsbHLH3 resulted in red pigmentation after 7 days, while no pigmentation was observed when PsMYB10.1 and PsbHLH3 were co-infiltrated with PsMYB18.【Conclusion】In this study, PsMYB18 was isolated and its expression was enhanced by the treatment at 20 ℃ and light. Phylogenetic and sequence analysis suggested that Pp MYB18 was likely a repressor of flavonoid biosynthesis. Transient color assay results showed that PsMYB18 was a negative regulator of anthocyanin biosynthesis.

MCLabX品牌 历史介绍:苏州蚂蚁淘生物科技有限公司,作为一家生命科学领域的高科技生物公司,目前代理销售二十多家欧美著名生物技术公司的产品,覆盖了免疫学、细胞生物学、分子生物学、药物筛选、生物制药、食品检测、疫苗生产等领域。


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