CN110779967A - 一种基于传统玻碳电极的NF-κB电化学检测方法 - Google Patents
一种基于传统玻碳电极的NF-κB电化学检测方法 Download PDFInfo
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Abstract
本发明属于分析化学技术领域,涉及一种基于传统玻碳电极的NF‑κB电化学检测方法。本发明主要是利用肽核酸(PNA)能够竞争性的结合含NF‑κB结合序列dsDNA中的互补ssDNA形成稳定的PNA‑DNA杂交链,NF‑κB的存在会抑制PNA‑DNA杂交链生成的原理。实验首先在激活的电极表面镀金并共价修饰PNA,PNA竞争性的结合含NF‑κB结合序列dsDNA中的互补ssDNA在电极表面形成稳定的PNA‑DNA杂交链,NF‑κB的存在会与dsDNA结合并抑制PNA‑DNA杂交链的形成且NF‑κB含量的差别会导致PNA‑DNA杂交链形成量不同,选取特异性嵌合于PNA‑DNA杂交链中MB作为电信号分子,利用差分脉冲伏安法测量NF‑κB不同浓度时MB的峰电流值,绘制NF‑κB浓度与峰电流值的关系曲线得出线性方程,通过检测电信号计算待测样品中NF‑κB含量。该方法灵敏度高,为NF‑κB的检测提供新思路。
Description
技术领域
本发明涉及一种基于传统玻碳电极的NF-κB电化学检测方法,属于分析化学领域。
背景技术
核转录因子NF-κB是隶属于锌指结构家族的转录因子,能与B细胞免疫球蛋白κ轻链启动子区域相结合,并且调控该区域基因启动表达的蛋白。NF-κB广泛存在于哺乳动物的各个细胞类型中,不同类型研究皆发现机体在健康状态和病理状态下NF-κB的表达量有明显的差异,NF-κB的含量变化在机体免疫、代谢、炎症反应、肿瘤发展以及其他病程的发生过程中发挥着重要的指示作用,对于疾病的发展、早期诊断或预防具有重要意义。因此,建立一种灵敏、快速、便捷检测NF-κB水平的方法是非常必要的。
现今,NF-κB的检测方法包括电泳迁移率变动分析,蛋白质免疫印迹等。然而,这些方法通常需要特异性抗体,繁琐的标记或特殊仪器。众所周知,标记过程往往是非常耗时且昂贵,甚至可能会导致生物分子的变性。电化学检测技术具有设备简单,价格低廉、灵敏度高、简便快捷,同时可以实现无标记检测等优点。其中玻璃碳电极具有化学稳定性高,热胀系数小,气密性好,可制成圆柱、圆盘电极形状等优点,在电化学实验中得到日益广泛的应用,近年来,被成功的应用于生物大分子定性或定量的检测。
发明内容
本发明的目的是发挥电化学检测技术的优势,建立一种简单、无需标记、成本低廉和高灵敏度的NF-κB检测方法。
本发明的技术方案:一种基于传统玻碳电极的NF-κB电化学检测方法,利用PNA与DNA的结合具有高亲和力与特异性,能够竞争性的结合dsDNA中的互补ssDNA形成稳定的PNA-DNA杂交链;MB能够嵌合于杂交双链,作为氧化还原指示剂放大电信号响应;设计了含有NF-κB结合序列的DNA,当NF-κB蛋白存在时,NF-κB蛋白与dsDNA的靶向结合能抑制PNA-DNA杂交链的生成,电极表面修饰的PNA单链与MB互作力不强,信号微弱;NF-κB含量的差别导致不同程度的信号响应,测得标准曲线,通过统计学分析得出NF-κB检测的线性方程并计算其含量。该方法具有良好的重复性,高的灵敏度,可应用于NF-κB的检测。
方法包括以下步骤:玻碳电极的预处理、金粒子修饰玻碳电极、PNA修饰镀金玻碳电极、样品与修饰电极共孵育、MB与修饰电极共孵育、NF-κB的电化学检测。
(1)玻碳电极的预处理
采用经典的预处理方式进行玻碳电极的预处理。具体步骤如下:用1、0.3μm的三氧化二粉末分别对直径为3mm圆盘玻碳电极进行抛光,之后用酒精和超纯水分别超声5min。之后将处理好的电极置于0.5M H2SO4中,在0V-1.5V电压范围内进行循环伏安扫描,扫速参数设置为0.1V/s,直至达到稳定后,室温干燥。
(2)金粒子修饰玻碳电极
将上述(1)中经过经典方法预处理的玻碳电极浸泡于5mL 2mM的氯金酸溶液(0.5MH2SO4溶解)中电沉积750s,沉积电位为-200mV。
(3)PNA修饰镀金玻碳电极
将上述(2)中镀金玻碳电极表面滴加0.5μM 5.0μL的PNA(0.1M PBS,pH=7.4),37℃孵育1.5h,蒸馏水冲洗。后将PNA修饰的电极置于100μL 1.0mM MCH溶液中30min进行占位去除非特异性吸附。
上述PNA的序列为:5′-Cys-ATG-GTC-GGG-ACT-TTC-CCT-3′。
(4)样品与修饰电极共孵育
对待测样品预处理:取12.5μL 0.06μM ssDNA1(0.1M PBS,0.25M NaCl,pH=7.4)与12.5μL 0.06μM ssDNA2(0.1M PBS,0.25M NaCl,pH=7.4),经90℃5min→70℃10min→50℃10min→30℃10min→10℃25min杂交得dsDNA。再与25μL不同浓度(0→0.1ng/mL)NF-κBp50(50mM HEPES,1mM TCEP,50mM NaCl,pH=7.4)溶液混合,37℃孵育0.5h。将经过上述(3)处理的电极置于dsDNA与蛋白的混合溶液中,37℃孵育2.0h。
上述ssDNA1的序列为:5′-ATG-GTC-GGG-ACT-TTC-CCT-3′;
上述ssDNA2的序列为:5′-AGG-GAA-AGT-CCC-GAC-CAT-3′
(5)MB与修饰电极共孵育
将经过上述(4)处理的电极置于100μL,浓度为20mM的MB溶液(20mM Tris-HCl,pH=7.4)中,避光,室温孵育2h。
(6)NF-κB的电化学检测
将经过上述(5)处理的电极置于5mL 20mM Tris-HCl,pH为7.4的溶液,进行电化学定量分析,本检测采用的电化学工作站(CHI 660E),以饱和甘汞电极为参比电极,铂电极为对电极。使用的扫描方法为微分脉冲伏安法,参数设置:初始电位-0.6V,终止电位0.3V,电位增量0.004V,振幅0.05V,脉冲宽度0.05s,脉冲周期0.5s。在NF-κB含量多的情况下,形成PNA-DNA的杂交链就越少,电信号分子MB吸附量就越少,因此得到的电化学信号也随之减小。以MB的电化学信号为纵坐标,NF-κB的浓度为横坐标,绘制标准曲线,通过计算NF-κB的浓度,即可实现NF-κB的灵敏检测。
本发明的有益效果:该方法简便快速、灵敏度高,成功实现了NF-κB的无标记检测。简化了实验步骤,避免了标记过程,对各类疾病包括癌症的监控与治疗具有重要意义。
附图说明
图1:NF-κB的检测原理图。
图2:NF-κB在不同浓度下,电化学信号值与NF-κB浓度关系的标准曲线图。
具体实施方式
实施例1.NF-κB标准溶液电化学信号值-浓度标准曲线图的测定
将25μL不同浓度NF-κB标准液分别按照上述步骤与DNA共孵育后修饰于电极,经电信号分子MB处理后测得电化学信号。如图2所示电化学信号值(ip)与NF-κB浓度的变化关系曲线,NF-κB在0.02-0.1ng/mL范围内,ip与浓度存在线性关系,线性回归方程为:y=-55.05x+7.101,R2=0.995,式中y为DPV的峰电流ip(μA),x为NF-κB的浓度(ng/mL)。
Claims (6)
1.一种基于传统玻碳电极的NF-κB电化学检测方法,其特征是利用肽核酸(PNA)能够竞争性的结合含NF-κB结合序列dsDNA中的互补ssDNA形成稳定的PNA-DNA杂交链,NF-κB的存在会抑制PNA-DNA杂交链生成的原理,实验首先在经处理的传统玻碳表面镀金并共价修饰PNA,PNA竞争性的结合含NF-κB结合序列dsDNA中的互补ssDNA在电极表面形成稳定的PNA-DNA杂交链,NF-κB的存在会与dsDNA结合并抑制PNA-DNA杂交链的形成且NF-κB含量的差别会导致PNA-DNA杂交链形成量不同,选取特异性嵌合于PNA-DNA杂交链中MB作为电信号分子,利用差分脉冲伏安法测量NF-κB不同浓度时MB的峰电流值,绘制NF-κB浓度与峰电流值的关系曲线得出线性方程,通过检测电信号计算待测样品中NF-κB含量。
2.根据权利要求1所述的一种基于传统玻碳电极的NF-κB电化学检测方法,其特征是利用PNA能够竞争性的结合含NF-κB结合序列dsDNA中的互补ssDNA形成稳定的PNA-DNA杂交链,NF-κB的存在会抑制PNA-DNA杂交链生成的原理。
3.根据权利要求1所述的一种基于传统玻碳电极的NF-κB电化学检测方法,其特征是实验首先在经处理的传统玻碳表面镀金并共价修饰PNA,该修饰过程首先通过经典方法预处理玻碳电极,之后将其浸泡于5mL 0.5M H2SO4溶解的浓度为2mM的氯金酸溶液中-200mV电沉积750s,双蒸水清洗后再于电极表面滴加5.0μL含0.5μM PNA、0.1M PBS,pH值为7.4的溶液,37℃孵育1.5h,蒸馏水冲洗后,于1mM巯基己醇溶液浸泡0.5h,蒸馏水冲洗,得到PNA稳定修饰的镀金玻碳电极表面。
4.根据权利要求1所述的一种基于传统玻碳电极的NF-κB电化学检测方法,其特征是PNA竞争性的结合含NF-κB结合序列dsDNA中的互补ssDNA在电极表面形成稳定的PNA-DNA杂交链,NF-κB的存在会与dsDNA结合并抑制PNA-DNA杂交链的形成且NF-κB含量的差别会导致PNA-DNA杂交链形成量不同,实验中取用0.25M NaCl、0.1M PBS,pH值为7.4溶液溶解的0.06μM ssDNA1与0.06μM ssDNA2各12.5μL混合,经90℃ 5min→70℃ 10min→50℃ 10min→30℃ 10min→10℃ 25min杂交得dsDNA,再将其与25μL用1mM TCEP、50mM NaCl、50mM HEPES,pH值7.4的溶液溶解NF-κB标准溶液混合,37℃孵育0.5h后,将权利要求2中的玻碳电极浸泡于该溶液中,37℃孵育2.0h。
5.根据权利要求1所述的一种基于传统玻碳电极的NF-κB电化学检测方法,其特征是是选取特异性嵌合于PNA-DNA杂交链中MB作为电信号分子,利用差分脉冲伏安法测量NF-κB不同浓度时MB的峰电流值,将权利要求4中的电极浸泡在100μL含20mM MB、20mM Tris-HCl,pH值为7.4的溶液中,室温避光孵育2h,双蒸水清洗后,将电极置于5mL 20 mM Tris-HCl,pH为7.4的溶液中进行差分脉冲伏安法分析,参数设置:初始电位-0.6V,终止电位0.3V,电位增量0.004V,振幅0.05V,脉冲宽度0.05s,脉冲周期0.5s。
6.根据权利要求1所述的一种基于传统玻碳电极的NF-κB电化学检测方法,其特征是绘制NF-κB浓度与峰电流值的关系曲线得出线性方程,通过检测电信号计算待测样品中NF-κB含量。
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