In breast cancer, a proper biomarker for the assessment of metastasis and poor prognosis is the RNA of activated leukocyte cell adhesion molecule (ALCAM) gene, which is expressed at high levels in breast tumor. We applied DNA-functionalized gold nanoparticles as the target-specific probes, for detecting specific sequences of DNA or RNA. At high MgCL2 concentrations, nanoprobes aggregate in the absence of the complementary DNA sequence and alteration in the solution color is detectable by evaluating the localized surface plasmon resonance (LSPR). But in the presence of complementary DNA, nanoprobes hybridize to the complementary sequence; therefore, no aggregation takes place, and no color change is observed. We designed a gold nanoprobe-based method that promptly detects the ALCAM gene expression in a low reaction volume with high sensitivity and specificity. This method is simple, fast, selective, and quantitative and can be done with small concentrations of the target (fmol/μL). Limit of detection of the method corresponded to 300 fmol/μL of synthetic ALCAM target.

译文

在乳腺癌中,用于评估转移和不良预后的适当生物标志物是活化的白细胞细胞粘附分子 (ALCAM) 基因的RNA,该RNA在乳腺肿瘤中高水平表达。我们使用DNA功能化的金纳米颗粒作为靶标特异性探针,用于检测DNA或RNA的特定序列。在高MgCL2浓度下,纳米探针在没有互补DNA序列的情况下聚集,并且通过评估局部表面等离子体共振 (LSPR) 可以检测到溶液颜色的改变。但是在存在互补DNA的情况下,纳米探针与互补序列杂交; 因此,没有发生聚集,也没有观察到颜色变化。我们设计了一种基于金纳米探针的方法,该方法可在低反应体积下以高灵敏度和特异性快速检测ALCAM基因表达。该方法简单,快速,选择性和定量,可以用小浓度的靶标 (fmol/μ l) 完成。该方法的检测限相当于合成ALCAM靶的300  fmol/μ l。

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