![Sample our Bioscience journals, sign in here to start your access, Latest two full volumes FREE to you for 14 days]({"type":"image" , "src" : "/sda/5925/TOC-Subject-Sample-2021-Bioscience.jpg"})
Abstract
The Sgs-7 and Sgs-8 glue genes at 68C are divergently transcribed and are separated by 475 bp. Fusion genes with Adh or lacZ coding sequences were constructed, and the expression of these genes, with different amounts of upstream sequences present, was tested by a transient expression procedure and by germ line transformation. A cis-acting element for both genes is located asymmetrically in the intergenic region between −211 and −43 bp relative to Sgs-7. It is required for correct expression of both genes. This element can confer the stageand tissue-specific expression pattern of glue genes on a heterologous promoter. An 86-bp portion of the element, from −133 to −48 bp relative to Sgs-7, is shown to be capable of enhancing the expression of a truncated and therefore weakly expressed Sgs-3 fusion gene. Recently described common sequence motifs of glue gene regulatory elements (T. Todo, M. Roark, K. Vijay Ragna van, C. A. Mayeda, and E. M. Meyerowitz, Mol. Cell. Biol. 10:5991−6002, 1990) are located within this 86-bp region.