Department of Biochemistry and Molecular Biology, Southern Illinois University School of Medicine, Carbondale, Illinois 62901.
Department of Biochemistry and Molecular Biology, Southern Illinois University School of Medicine, Carbondale, Illinois 62901
Genetics. 2018 Jan;208(1):191-205. doi: 10.1534/genetics.117.300518. Epub 2017 Nov 15.
SAGA (Spt-Ada-Gcn5-Acetyltransferase) and TFIID (transcription factor IID) have been previously shown to facilitate the formation of the PIC (pre-initiation complex) at the promoters of two distinct sets of genes. Here, we demonstrate that TFIID and SAGA differentially participate in the stimulation of PIC formation (and hence transcriptional initiation) at the promoter of , a gene for the high-affinity inorganic phosphate (P) transporter for crucial cellular functions, in response to nutrient signaling. We show that transcriptional initiation of occurs predominantly in a TFIID-dependent manner in the absence of P in the growth medium. Such TFIID dependency is mediated via the NuA4 (nucleosome acetyltransferase of H4) histone acetyltransferase (HAT). Intriguingly, transcriptional initiation of also occurs in the presence of P in the growth medium, predominantly via the SAGA complex, but independently of NuA4 HAT. Thus, P in the growth medium switches transcriptional initiation of from NuA4-TFIID to SAGA dependency. Further, we find that both NuA4-TFIID- and SAGA-dependent transcriptional initiations of are facilitated by the 19S proteasome subcomplex or regulatory particle (RP) via enhanced recruitment of the coactivators SAGA and NuA4 HAT, which promote TFIID-independent and -dependent PIC formation for transcriptional initiation, respectively. NuA4 HAT does not regulate activator binding to , but rather facilitates PIC formation for transcriptional initiation in the absence of Pi in the growth medium. On the other hand, SAGA promotes activator recruitment to for transcriptional initiation in the growth medium containing Pi. Collectively, our results demonstrate two distinct stimulatory pathways for PIC formation (and hence transcriptional initiation) at by TFIID, SAGA, NuA4, and 19S RP in the presence and absence of an essential nutrient, P, in the growth media, thus providing new regulatory mechanisms of transcriptional initiation in response to nutrient signaling.
SAGA(SpT-Ada-Gcn5-Acetyltransferase)和 TFIID(转录因子IID)先前已被证明可促进两组不同基因启动子处 PIC(起始前复合物)的形成。在这里,我们证明 TFIID 和 SAGA 以不同的方式参与在营养信号响应中,对于关键细胞功能的高亲和力无机磷酸盐(P)转运体基因 的启动子处 PIC 形成(因此转录起始)的刺激。我们表明,在生长培养基中没有 P 的情况下, 基因的转录起始主要以 TFIID 依赖的方式发生。这种 TFIID 依赖性是通过 NuA4(H4 核小体乙酰转移酶)组蛋白乙酰转移酶(HAT)介导的。有趣的是,在生长培养基中有 P 的情况下, 基因的转录起始也主要通过 SAGA 复合物发生,但不依赖于 NuA4 HAT。因此,生长培养基中的 P 将 的转录起始从 NuA4-TFIID 切换到 SAGA 依赖性。此外,我们发现,NuA4-TFIID-和 SAGA 依赖性的 基因转录起始都通过 19S 蛋白酶体亚基或调节颗粒(RP)得到促进,通过增强共激活因子 SAGA 和 NuA4 HAT 的募集,分别促进 TFIID 非依赖性和依赖性 PIC 的形成,从而促进转录起始。NuA4 HAT 不调节激活剂与 基因的结合,但在生长培养基中没有 Pi 的情况下,它促进 PIC 形成以进行转录起始。另一方面,SAGA 促进激活剂募集到含有 Pi 的生长培养基中的 基因以进行转录起始。总的来说,我们的结果表明,在生长培养基中存在和不存在必需营养素 P 的情况下,通过 TFIID、SAGA、NuA4 和 19S RP,存在两种不同的刺激途径来促进 PIC 的形成(因此转录起始),从而为营养信号响应中的转录起始提供了新的调控机制。
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