21 research outputs found
Epigenomic Comparison Reveals Activation of âSeedâ Enhancers during Transition from Naive to Primed Pluripotency
SummaryNaive mouse embryonic stem cells (mESCs) and primed epiblast stem cells (mEpiSCs) represent successive snapshots of pluripotency during embryogenesis. Using transcriptomic and epigenomic mapping we show that a small fraction of transcripts are differentially expressed between mESCs and mEpiSCs and that these genes show expected changes in chromatin at their promoters and enhancers. Unexpectedly, the cis-regulatory circuitry of genes that are expressed at identical levels between these cell states also differs dramatically. In mESCs, these genes are associated with dominant proximal enhancers and dormant distal enhancers, which we term seed enhancers. In mEpiSCs, the naive-dominant enhancers are lost, and the seed enhancers take up primary transcriptional control. Seed enhancers have increased sequence conservation and show preferential usage in downstream somatic tissues, often expanding into super enhancers. We propose that seed enhancers ensure proper enhancer utilization and transcriptional fidelity as mammalian cells transition from naive pluripotency to a somatic regulatory program
Identification and Characterization of Cell TypeâSpecific and Ubiquitous Chromatin Regulatory Structures in the Human Genome
The identification of regulatory elements from different cell types is necessary for understanding the mechanisms controlling cell typeâspecific and housekeeping gene expression. Mapping DNaseI hypersensitive (HS) sites is an accurate method for identifying the location of functional regulatory elements. We used a high throughput method called DNase-chip to identify 3,904 DNaseI HS sites from six cell types across 1% of the human genome. A significant number (22%) of DNaseI HS sites from each cell type are ubiquitously present among all cell types studied. Surprisingly, nearly all of these ubiquitous DNaseI HS sites correspond to either promoters or insulator elements: 86% of them are located near annotated transcription start sites and 10% are bound by CTCF, a protein with known enhancer-blocking insulator activity. We also identified a large number of DNaseI HS sites that are cell type specific (only present in one cell type); these regions are enriched for enhancer elements and correlate with cell typeâspecific gene expression as well as cell typeâspecific histone modifications. Finally, we found that approximately 8% of the genome overlaps a DNaseI HS site in at least one the six cell lines studied, indicating that a significant percentage of the genome is potentially functional
Speeding to Pluripotency
Finding a cell that reprograms in a nonstochastic manner without genetic manipulation has proven elusive. In this issue, Guo et al. report the identification of a cell defined by an ultrafast cycle whose progeny reprogram in a synchronous and rapid manner
Sox2 Acts through Sox21 to Regulate Transcription in Pluripotent and Differentiated Cells
SummarySox2 is an important transcriptional regulator in embryonic and adult stem cells [1â4]. Recently, Sox2 was identified as an oncogene in many endodermal cancers, including colon cancer [5â8]. There is great interest in how Sox2 cooperates with other transcription factors to regulate stem cell renewal, differentiation, and reprogramming [9]. However, we still lack a general understanding of Sox2 transcriptional action. To determine transcriptional partners of Sox2 in adult cells, we generated mice where gene expression could be induced by an externally applied stimulus. We analyzed the consequences in the intestine where cell turnover is rapid. Sox2 expression, but not Oct4, specifically increased the numbers of stem cells and repressed Cdx2, a master regulator of endodermal identity. In vivo studies demonstrated that Sox21, another member of the SoxB gene family, was a specific, immediate, and cell-autonomous target of Sox2 in intestinal stem cells. In vitro experiments showed that Sox21 was sufficient to repress Cdx2 in colon cancer cells and in pluripotent stem cells. Sox21 was also specifically induced by Sox2 in fibroblasts and inhibition of Sox21 blocked reprogramming to the pluripotent state. These results show that transcriptional induction of Sox21 is a rapid and general mediator of the effects of Sox2 on cell identity in a wide range of cell types
Concise Review: Reprogramming, Behind the Scenes: Noncanonical Neural Stem Cell Signaling Pathways Reveal New, Unseen Regulators of Tissue Plasticity With Therapeutic Implications
Interest is great in the new molecular concepts that explain, at the
level of signal transduction, the process of reprogramming. Usually,
transcription factors with developmental importance are used, but these
approaches give limited information on the signaling networks involved,
which could reveal new therapeutic opportunities. Recent findings
involving reprogramming by genetic means and soluble factors with
well-studied downstream signaling mechanisms, including signal
transducer and activator of transcription 3 (STAT3) and hairy and
enhancer of split 3 (Hes3), shed new light into the molecular mechanisms
that might be involved. We examine the appropriateness of common culture
systems and their ability to reveal unusual (noncanonical) signal
transduction pathways that actually operate in vivo. We then discuss
such novel pathways and their importance in various plastic cell types,
culminating in their emerging roles in reprogramming mechanisms. We also
discuss a number of reprogramming paradigms (mouse induced pluripotent
stem cells, direct conversion to neural stem cells, and in vivo
conversion of acinar cells to beta-like cells). Specifically for
acinar-to-beta-cell reprogramming paradigms, we discuss the common view
of the underlying mechanism (involving the Janus kinase-STAT pathway
that leads to STAT3-tyrosine phosphorylation) and present alternative
interpretations that implicate STAT3-serine phosphorylation alone or
serine and tyrosine phosphorylation occurring in sequential order. The
implications for drug design and therapy are important given that
different phosphorylation sites on STAT3 intercept different signaling
pathways. We introduce a new molecular perspective in the field of
reprogramming with broad implications in basic, biotechnological, and
translational research
Use of postmortem human dura mater and scalp for deriving human fibroblast cultures.
Fibroblasts can be collected from deceased individuals, grown in culture, reprogrammed into induced pluripotent stem cells (iPSCs), and then differentiated into a multitude of cell types, including neurons. Past studies have generated iPSCs from somatic cell biopsies from either animal or human subjects. Previously, fibroblasts have only been successfully cultured from postmortem human skin in two studies. Here we present data on fibroblast cell cultures generated from 146 scalp and/or 53 dura mater samples from 146 postmortem human brain donors. In our overall sample, the odds of successful dural culture was almost two-fold compared with scalp (OR = 1.95, 95% CI: [1.01, 3.9], p = 0.047). Using a paired design within subjects for whom both tissues were available for culture (n = 53), the odds of success for culture in dura was 16-fold as compared to scalp (OR = 16.0, 95% CI: [2.1-120.6], p = 0.0007). Unattended death, tissue donation source, longer postmortem interval (PMI), and higher body mass index (BMI) were associated with unsuccessful culture in scalp (all p<0.05), but not in dura. While scalp cells proliferated more and grew more rapidly than dura cells [F (1, 46) = 12.94, p<0.008], both tissues could be generated and maintained as fibroblast cell lines. Using a random sample of four cases, we found that both postmortem scalp and dura could be successfully reprogrammed into iPSC lines. Our study demonstrates that postmortem dura mater, and to a lesser extent, scalp, are viable sources of living fibroblasts for culture that can be used to generate iPSCs. These tissues may be accessible through existing brain tissue collections, which is critical for studying disorders such as neuropsychiatric diseases
Demographic and sample parameters of successful culture in scalp (nâ=â146).
<p>ORâ=âodds ratio, AAâ=âAfrican-American, Wâ=âWhite, PMIâ=âpostmortem interval, BMIâ=âbody mass index, Fâ=âfemale, Mâ=âmale, VAâ=âVirginia, DCâ=âDistrict of Columbia; Toxâ=âtoxicology testing in blood or vitreous humor; *â=âp<0.05.</p
Fibroblast characterization: FSP-1 protein expression by immunofluorescence staining and cell proliferation assay in dura and scalp. A.
<p>The morphology of postmortem fibroblast cells generated from (a) dura and (b) scalp. Cultured cells from both sources macroscopically looked similar to what is seen in living skin fibroblast cells, with more enriched cytoplasm and spindle-shaped nuclei under phase-contrast microscopy. Cells from (c) dura and (d) scalp express cytoplasmic Fibroblast Specific Protein-1 (FSP-1) (green). Original scale barsâ=â35 ”m. <b>B.</b> Results from cell proliferation assay in 8 fibroblast cell lines (dura and scalp from 4 individuals) in five different densities. Cell viability was determined in 24 hrs and 48 hrs by WST-8 assay. Values are the mean of results from six wells. Bars ± SE. Scalp fibroblast cell lines grew 1.27-fold faster in the same period than dura fibroblast cells. <b>C.</b> Differences in cell proliferation between scalp and dura by one-way ANOVA; scalp cell growth was significantly more rapid than dura cell growth at 24 hr and 48 hr intervals [F (1, 46)â=â12.94, p<0.008].</p