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-Subunit Glycoprotein Hormone Promoter with Trophoblast Specificity and Maximal Activity
Department of Pharmacology (P.R.B., J.H.N.), School of
Medicine, Case Western Reserve University, Cleveland, Ohio
44106,
Department of Cellular and Molecular Physiology
(P.G.Q.), The Pennsylvania State University College of Medicine,
Hershey, Pennsylvania 17033
Trophoblast-specific expression of the human
-subunit glycoprotein hormone gene requires a tightly linked array
of five different regulatory elements [trophoblast-specific element
(TSE),
-activating element (
ACT), a tandem cAMP response element
(CRE), junctional regulatory element (JRE), and a CCAAT box]. We
examined their contextual contributions to trophoblast-specific
expression by using transfection assays to evaluate activity of
systematic block replacement mutations made within the 1500-bp
5'-flanking region of the human
-subunit gene. While all five
elements were required for full activity, only the TSE and JRE
displayed trophoblast specificity. Interestingly, the TSE-binding
protein has limited tissue distribution whereas a JRE-binding protein
appears trophoblast specific. Likewise, replacement studies with an
AP-1 element that binds heterodimers of jun and
fos indicated that this element was incapable of
compensating for either the tandem CRE or JRE. This preference for both
CRE- and JRE-binding proteins provides another avenue for configuring
an
-subunit promoter with trophoblast specificity. Additional
analysis with a cAMP response element binding protein (CREB)-Gal4
fusion protein further underscored the importance of CREB as well as
suggested that transcriptional contributions come from both the
DNA-binding domain and transactivation domain of this protein. We also
examined the interactive nature of the pentameric array by placing a
15-bp random sequence between each element. Remarkably, only the
insertion 3' of the CCAAT box diminished promoter activity. This
suggested the absence of direct interactions between the
transcriptional factors that bind each element in the array. It also
suggested that the CCAAT box is position-dependent relative to the TATA
box. This position dependence appeared cell-specific, as it was not
manifest in a gonadotrope cell line (
T31 cells). Thus, the CCAAT
box also has tissue-specific characteristics that assist in targeting
expression of the
-subunit gene to trophoblasts. Together, these
data suggest that multiple characteristics of a complex pentameric
array of regulatory elements endow the
-subunit promoter with
trophoblast specificity and maximal activity.
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