• Journal of the Korean Wood Science and Technology
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• 제35권4호
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• pp.52-60
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• 2007

포르말린과 톨루엔 처리에 의한 애기장대의 표현형 변화 및 포르말린에 의한 단백질의 발현변화를 관찰하였다. 톨루엔의 휘발량이 포르말린보다 많음에도 불구하고 포르말린 처리구에서 애기장대의 표현형 변화가 더욱 현저한 것을 확인하였다. 포르말린에 의한 표현형의 변화가 미비한 6h 처리구에서도 애기장대 단백질의 발현에 많은 변화가 나타났으며 이러한 발현변화는 처리시간이 길어질수록 더욱 뚜렷하였다. 포르말린에 의하여 발현량이 변하는 단백질의 분자량을 automated gel electrophoresis system을 이용하여 예측한 후, 그 결과를 토대로 formaldehyde-responsive proteins을 분리하였다. 분리한 5개의 단백질은 전사수준에서 formaldehyde-dependent expression을 나타내었으며 formaldehyde-responsive proteins (FRP)으로 명명하였다. FRP5를 제외한 네 개의 단백질은 그 기능이 밝혀지지 않은 novel protein으로 식물의 방어기작에 관여하는 단백질과 높은 상동성을 나타내는 것을 알 수 있었다.

• 대한의생명과학회지
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• 제14권1호
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• pp.47-53
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• 2008

Hox genes are known to be transcription factors controlling vertebrate pattern formation along the anteroposterior body axis by regulating many target gene expressions during vertebrate embryogenesis. In order to isolate in vivo Hox responsive target genes, ChIP-cloning technique has been applied using Hoxc8 antibody. Here murine embryo of day 11.5 post coitum (E11.5) highly expressing Hoxc8 gene was used after removing head and tail portions where Hoxc8 is rarely expressing. After fixation with formaldehyde, the chromatin DNAs harboring bound proteins were isolated. After sonication, about 0.5- to 1 Kb chromatin DNAs were immunoprecipitated with anti Hoxc8 antibody. After removing the bound proteins with proteinase K, DNAs were isolated, cloned into the pBluescsript II SK vector, and then sequenced. Total 33 random clones sequenced were anlalyzed to be located at 12 different genomic regions. Among these, 8 turned out to be introns and 4 were intergenic regions localized in random chromosomes. The base composition of total cloned genomic sequences (6608 bp) were AT-rich, i.e., 40% GC. When the Hoxc8 core binding sites, such as TAAT, ATTA, TTAT, and ATAA were analyzed total number of 55, 45, 54, and 55 were found, respectively, which are than twice as many as expected number of 26. Although this in silico analysis does not mean that the ChIP-cloned sequence is real Hoxc8 regulatory element in vivo, these results strongly imply that the DNA fragments cloned through chromatin immunoprecipitation could be very much likely the putative Hoxc8 downstream target genes.