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表面化学和封闭策略对DNA微阵列的影响。

Impact of surface chemistry and blocking strategies on DNA microarrays.

作者信息

Taylor Scott, Smith Stephanie, Windle Brad, Guiseppi-Elie Anthony

机构信息

Center for Bioelectronics, Biosensors and Biochips (C3B), Virginia Commonwealth University, PO Box 843038, 601 West Main Street, Richmond, VA 23284-3038, USA.

出版信息

Nucleic Acids Res. 2003 Aug 15;31(16):e87. doi: 10.1093/nar/gng086.

Abstract

The surfaces and immobilization chemistries of DNA microarrays are the foundation for high quality gene expression data. Four surface modification chemistries, poly-L-lysine (PLL), 3-glycidoxypropyltrimethoxysilane (GPS), DAB-AM-poly(propyleminime hexadecaamine) dendrimer (DAB) and 3-aminopropyltrimethoxysilane (APS), were evaluated using cDNA and oligonucleotide sub-arrays. Two un-silanized glass surfaces, RCA-cleaned and immersed in Tris-EDTA buffer were also studied. DNA on amine-modified surfaces was fixed by UV (90 mJ/cm(2)), while DNA on GPS-modified surfaces was immobilized by covalent coupling. Arrays were blocked with either succinic anhydride (SA), bovine serum albumin (BSA) or left unblocked prior to hybridization with labeled PCR product. Quality factors evaluated were surface affinity for cDNA versus oligonucleotides, spot and background intensity, spotting concentration and blocking chemistry. Contact angle measurements and atomic force microscopy were preformed to characterize surface wettability and morphology. The GPS surface exhibited the lowest background intensity regardless of blocking method. Blocking the arrays did not affect raw spot intensity, but affected background intensity on amine surfaces, BSA blocking being the lowest. Oligonucleotides and cDNA on unblocked GPS-modified slides gave the best signal (spot-to-background intensity ratio). Under the conditions evaluated, the unblocked GPS surface along with amine covalent coupling was the most appropriate for both cDNA and oligonucleotide microarrays.

摘要

DNA微阵列的表面及固定化学性质是高质量基因表达数据的基础。使用cDNA和寡核苷酸子阵列评估了四种表面修饰化学方法,即聚-L-赖氨酸(PLL)、3-缩水甘油氧基丙基三甲氧基硅烷(GPS)、DAB-AM-聚(丙胺十六胺)树枝状聚合物(DAB)和3-氨丙基三甲氧基硅烷(APS)。还研究了两种未硅烷化的玻璃表面,即经过RCA清洗并浸入Tris-EDTA缓冲液中的表面。胺修饰表面上的DNA通过紫外线(90 mJ/cm²)固定,而GPS修饰表面上的DNA通过共价偶联固定。在与标记的PCR产物杂交之前,阵列用琥珀酸酐(SA)、牛血清白蛋白(BSA)封闭或不封闭。评估的质量因素包括cDNA与寡核苷酸的表面亲和力、斑点和背景强度、点样浓度和封闭化学方法。进行接触角测量和原子力显微镜检查以表征表面润湿性和形态。无论封闭方法如何,GPS表面的背景强度最低。封闭阵列不影响原始斑点强度,但会影响胺表面的背景强度,BSA封闭时背景强度最低。未封闭的GPS修饰载玻片上的寡核苷酸和cDNA产生的信号最佳(斑点与背景强度比)。在所评估的条件下,未封闭的GPS表面与胺共价偶联最适合cDNA和寡核苷酸微阵列。

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