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        Generation of cDNA Libraries for Profiling Gene Expression of Given Tissues or Cells

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        Complementary DNA (cDNA) library construction is a foundational technique for various organism genome projects and molecular biological approaches. Numerous methods for generating a cDNA library have been applied for different purposes. To profile the gene expression of a given tissue or cells, the researchers often used an oligo-(dT) primed and directional cloned strategy for generating cDNA libraries, and then DNA sequencing to characterize novel genes from those libraries (1 6 ). The cDNA library derived from the strategy may contain more abundance gene species without significant bias because polymerase chain reaction (PCR) is not usually used for amplifying the double-strain cDNA. However, the strategy needs more sample and abundant message RNA. If there is only a little mRNA, the PCR-based method must been adopted in cDNA library construction. Recently, some researchers utilized cap structure at the 5′ end of eukaryotic mRNA to design novel methods for PCR-based cDNA library construction (7 11 ). Moreover, the strategy has been applied to identifying gene expression and isolating full-length cDNA (12 14 ). In our laboratory, the conventional and PCR-based strategies have been utilized for generating some libraries from massive sample (human liver cancer, hypothalamus, pituitary, adrenal gland) and a small amount of RNA (human CD34+ cells), respectively.
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