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Enzyme microarrays assembled by acoustic dispensing technology

机译:通过声学分配技术组装的酶微阵列

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摘要

Miniaturizing bioassays to the nanoliter scale for high-throughput screening reduces the consumption of reagents that are expensive or difficult to handle. Through the use of acoustic dispensing technology, nanodroplets containing 10 μM ATP (3 μCi/μL 32P) and reaction buffer in 10% glycerol were positionally dispensed to the surface of glass slides to form 40-nL compartments (100 droplets/slide) for Pim1 (proviral integration site 1) kinase reactions. The reactions were activated by dispensing 4 nL of various levels of a pyridocarbazolo-cyclopentadienyl ruthenium complex Pim1 inhibitor, followed by dispensing 4 nL of a Pim1 kinase and peptide substrate solution to achieve final concentrations of 150 nM enzyme and 10 μM substrate. The microarray was incubated at 30 °C (97% Rh) for 1.5 h. The spots were then blotted to phosphocellulose membranes to capture phosphorylated substrate. With phosphor imaging to quantify the washed membranes, the assay showed that, for doses of inhibitor from 0.75 to 3 μM, Pim1 was increasingly inhibited. Signal-to-background ratios were as high as 165, and average coefficients of variation for the assay were not, vert, ∼20%. Coefficients of variation for dispensing typical working buffers were under 5%. Thus, microarrays assembled by acoustic dispensing are promising as cost-effective tools that can be used in protein assay development.
机译:用于高通量筛选的将生物测定微型化至纳升规模可减少昂贵或难以处理的试剂的消耗。通过使用声学点胶技术,将含有10μMATP(3μCi/μL32P)和10%甘油中的反应缓冲液的纳米液滴按位置分配到载玻片的表面,以形成用于Pim1的40 nL隔室(每滴100滴)。 (附加整合位点1)激酶反应。通过分配4 nL各种水平的吡啶并咔唑-环戊二烯基钌复合物Pim1抑制剂来激活反应,然后分配4 nL的Pim1激酶和肽底物溶液以达到150 nM酶和10μM底物的最终浓度。将微阵列在30°C(97%Rh)下孵育1.5小时。然后将斑点印迹到磷酸纤维素膜上以捕获磷酸化的底物。通过荧光粉成像来量化清洗过的膜,该分析表明,对于0.75至3μM的抑制剂剂量,Pim1被越来越多地抑制。信噪比高达165,该分析的平均变异系数未达到〜20%。分配典型工作缓冲液的变异系数低于5%。因此,通过声学分配组装的微阵列有望成为可用于蛋白质测定开发的经济有效的工具。

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