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151. Demonstration of Rabies Viral Nucleic Acids by In-Situ Polymerase Chain Reaction

152. Deterministic Whole-Genome Amplification of Single Cells

153. Real-Time PCR Approaches for Analysis of Hydrocarbon-Degrading Bacterial Communities

154. The Utility of Whole Genome Amplification for Typing Compromised Forensic Samples

155. Primer design for multiplex PCR using a genetic algorithm

156. Reliable amplification method for bacterial RNA

157. Real-time PCR: A review of approaches to data analysis

158. APPLICATION OF NUCLEIC ACID SEQUENCE-BASED AMPLIFICATION FOR THE DETECTION OF VIABLE FOODBORNE PATHOGENS: PROGRESS AND CHALLENGES

159. Amplification of chloroplast DNA using the polymerase chain reaction (PCR): a practical activity for secondary school students

160. An efficient and economic enhancer mix for PCR

161. Circumventing air bubbles in microfluidic systems and quantitative continuous-flow PCR applications

162. Selection of aptamers by systematic evolution of ligands by exponential enrichment: Addressing the polymerase chain reaction issue

163. Amplification of circularizable probes for the detection of target nucleic acids and proteins

164. Noninvasive genetic sampling of endangered muriqui (Primates, Atelidae): efficiency of fecal DNA extraction

165. Nucleic acid amplification-based techniques for pathogen detection and identification

166. The Polymerase Chain Reaction (PCR): Solution PCR on Paraffin–Embedded Human Tissues

167. A protocol for high-throughput extraction of DNA from rice leaves

168. Quantitative real-time RT-PCR – a perspective

169. Similar sequence-free amplification of human glyceraldehyde-3-phosphate dehydrogenase for real time RT-PCR applications

170. Improving Health Care and Laboratory Medicine: The Past, Present, and Future of Molecular Diagnostics

171. Polymerase chain reaction analysis of transgenic plants contaminated byAgrobacterium

172. Overcoming bacterial DNA contamination in real-time PCR and RT-PCR reactions for LacZ detection in cell therapy monitoring

173. Oligonucleotides used as template calibrators for general application in quantitative polymerase chain reaction

174. DNA amplification method tolerant to sample degradation

175. Isothermal whole genome amplification from single and small numbers of cells: a new era for preimplantation genetic diagnosis of inherited disease

176. Direct and Repeat Uses of Tissue Sections as Templates for Liquid-phase Polymerase Chain Reaction Amplification

177. Helicase‐dependent isothermal DNA amplification

178. Isothermal Multiple Displacement Amplification

179. Comparison of primers for the detection of Salmonella enterica serovars using real-time PCR

180. Use of multiple displacement amplification to amplify genomic DNA before sequencing of the and haemoglobin genes

181. Nucleic Acid Amplification Strategies for DNA Microarray-Based Pathogen Detection

182. A novel strategy to engineer DNA polymerases for enhanced processivity and improved performance in vitro

183. Pre-PCR Processing : Strategies to Generate PCR-Compatible Samples

184. Fluorescent in situ sequencing on polymerase colonies

185. PROBEmer: a web-based software tool for selecting optimal DNA oligos

186. Polymerase chain reaction and its applications

187. Avoiding false positives in PCR-based identification methods for nonsterile plant pathogens

188. Isothermal reactions for the amplification of oligonucleotides

189. Optimisation of PCR reactions using primer chessboarding

190. Broad-Range Ribosomal RNA Real-Time PCR after Removal of DNA from Reagents: Melting Profiles for Clinically Important Bacteria

191. Applications of polymerase chain reaction in rheumatology

192. [Untitled]

193. Isothermal Strand-Displacement Amplification Applications for High-Throughput Genomics

194. Influence of reagents formulation on real-time PCR parameters

195. TempliPhi, ⌽29 DNA Polymerase Based Rolling Circle Amplification of Templates for DNA Sequencing

196. Comprehensive human genome amplification using multiple displacement amplification

197. A Whole Genome Amplification Method to Generate Long Fragments from Low Quantities of Genomic DNA

198. Gene Specific-Primer Extension Preamplification (GS-PEP), a simple method to increase the copy number of a gene prior to PCR amplification

199. Correction: Examining Sources of Error in PCR by Single-Molecule Sequencing

200. Examining Sources of Error in PCR by Single-Molecule Sequencing

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