Detection of Endogenous K-ras mRNA in Living Cells at a Single Base Resolution by a PNA Molecular Beacon

被引:79
作者
Kam, Yossi [1 ]
Rubinstein, Abraham [1 ,2 ,3 ]
Nissan, Aviram [4 ]
Halle, David [4 ]
Yavin, Eylon [1 ]
机构
[1] Hebrew Univ Jerusalem, Fac Med, Sch Pharm, Inst Drug Res, IL-91120 Jerusalem, Israel
[2] Hebrew Univ Jerusalem, Fac Sci, Harvey M Krueger Family Ctr Nanosci & Nanotechnol, IL-91904 Jerusalem, Israel
[3] Hebrew Univ Jerusalem, Sch Pharm, Fac Med, David R Bloom Ctr Pharm, IL-91120 Jerusalem, Israel
[4] Hadassah Hebrew Univ, Med Ctr, Dept Surg, IL-91240 Jerusalem, Israel
关键词
hybridization; in vivo imaging; KRAS oncogene; molecular beacon; mRNA; peptide nucleic acids; PEPTIDE NUCLEIC-ACIDS; REAL-TIME DETECTION; PROBES FIT-PROBES; FLUOROGENIC PROBES; COLORECTAL-CANCER; GENE-EXPRESSION; DNA; DELIVERY; HYBRIDIZATION; FLUORESCENCE;
D O I
10.1021/mp200505k
中图分类号
R-3 [医学研究方法]; R3 [基础医学];
学科分类号
1001 ;
摘要
Detection of mRNA alterations is a promising approach for identifying biomarkers as means of differentiating benign from malignant lesions. By choosing the KRAS oncogene as a target gene, two types of molecular beacons (MBs) based on either phosphothioated DNA (PS-DNA-MB) or peptide nucleic acid (TO-PNA-MB, where TO = thiazole orange) were synthesized and compared in Vitro and in vivo. Their specificity was examined in wildtype KRAS (HT29) or codon 12 point mutation (Panc-1, SW480) cells. Incubation of both beacons with total RNA extracted from the Panc-1 cell line (fully complementary sequence) showed a fluorescent signal for both beacons. Major differences were observed, however, for single mismatch mRNA transcripts in cell lines HT29 and SW480. PS-DNA-MB weakly discriminated such single mismatches in comparison to TO-PNA-MB, which was profoundly more sensitive. Cell transfection of TO-PNA-MB with the aid of PEI resulted in fluorescence in cells expressing the fully complementary RNA transcript (Panc-1) but undetectable fluorescence in cells expressing the K-ras mRNA that has a single mismatch to the designed TO-PNA-MB (HT29). A weaker fluorescent signal was also detected in SW480 cells; however, these cells express approximately one-fifth of the target mRNA of the designed TO-PNA-MB. In contrast, PS-DNA-MB showed no fluorescence in all cell lines tested post PEI transfection. Based on the fast hybridization kinetics and on the single mismatch discrimination found for TO-PNA-MB we believe that such molecular beacons are promising for in vivo real-time imaging of endogenous mRNA with single nucleotide polymorphism (SNP) resolution.
引用
收藏
页码:685 / 693
页数:9
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