The evolution of codon usage and base composition

Perry, Richard Henry John

January 2015

This thesis aims to address issues relating to genome architecture and base composition. The first part of this thesis addresses questions relating to codon usage. Initially I will investigate thousands of bacterial species using a detailed analysis of strengths of selection acting upon codons usage while also investigating patterns of optimal codon changes with respect to genomic base composition and tRNA abundance. I report that selection on codon usage increases throughout the length of highly expressed genes, in particular, the first quarter of genes have significantly lower selection. Further, it is clear that factors affecting genomic base composition can eventually lead to changes in optimal codons if the change in base composition is strong enough, however these patterns differ substantially between amino acids. The debate over translational efficiency vs. accuracy was addressed by comparing sites of differing conservation. Differing conservation were defined using a phylogenetic method, allowing sites to change in their extent of conservation throughout the tree. The results show that translational accuracy acts strongly on the top 10% of conserved sites, however is relatively weak when compared to the efficiency for other sites. Also detected is a reduction in apparent selection on codon usage on the bottom 10% of conserved sites which is likely to be caused by conflicting positive selection on amino acids. Finally, although differences in patterns are observed between amino acids, the general relationship to conservation is similar. As much of the variation in codon usage is determined by variation in base composition, this aspect of base composition is investigated in the second part of the thesis. The observed variation in intragenomic base composition in bacteria was found to be far higher than expected for GC-rich bacteria. The non-core part of the genome contributes to this variation to a greater extent than the core part, suggesting that processes such as AT-rich horizontal gene transfer may be involved. Secondly, base composition is modelled under Brownian motion and as an extension, the Ornstein- Uhlenbeck process, which allows for multiple optima throughout the tree. The model including optima fits the data better than standard Brownian motion or Brownian motion with multiple diffusion coefficients. Finally, I investigate a case where a previous codon usage analysis has been seriously confounded by an unusual genome architecture of abnormal regional base composition in two species of eukaryotic parasites in the genus Theileria. In both species, the background G+C content is 37% at most, out of the four syntenic chromosomes. In many orthologous regions however, T.annulata has a decreased G+C content of 28% while T.parva has an increased G+C content of 41%. Various factors coincide with this remarkable divergence: increased divergence at all types of site, recombination hot spots in T.parva, an increased frequency of tandem repeats and DNA sequence motifs in both species. The evolutionary origins of these unusual patterns will be discussed.

572.8

The role of MuB in selecting transposition targets of bacteriophage Mu

Ge, Jun

19 January 2011

Bacteriophage Mu exhibits low specificity for the 5 bp sequence it selects as its transposition target, but shows regional biases in its insertion choices. For example, Mu prefers AT-rich DNA in vitro, exhibits a 1000-fold bias in target preference within the E. coli chromosome, and avoids targets carrying Mu end sequences. The Mu transposase is responsible for recognition of the 5 bp target consensus, but depends on the accessory protein MuB for efficient target capture. MuB preferentially binds to AT-rich DNA, explaining this particular regional preference. We have uncovered opposing roles for MuB in target capture and integration. We show while MuB-bound AT-rich DNA is favored for integration, the bound DNA itself is refractory, and that transposition occurs adjacent to, but not within the bound region. We show that this property of MuB is likely responsible for immunity of Mu from self-integration, since MuB was found to be strongly bound within the Mu genome. Genome-wide analysis of MuB binding on the E. coli chromosome showed that Mu target preference is positively related to MuB binding profile, and that MuB binding is insulated by the nucleoid-associated protein Fis but not by transcription events. Since Fis binding to the chromosome responds to the frequency of A-tracts, a chromosome domain structure signal, Mu transposition must also respond to chromosome domain signals. Work in this dissertation has provided a new understanding of how MuB influences and controls Mu target choice, and of reciprocal interactions between a bacterial chromosome and a transposable element. / text

Mu transposase

5 bp target consensus

Protein MuB

AT-rich DNA

Mu genome

Territórios heterocromáticos em Triatoma infestans Klug e Panstrongylus megistus (Burmeister) = composição, identificação de marcadores epigenéticos e resposta a inibidores de deacetilases de histonas / Heterochromatic territories in Triatoma infestans Klug and Panstrongylus megistus (Burmeister) : composition, identification of epigenetic markers and response to histone deacetylase inhibitors

Alvarenga, Elenice Monte, 1988-

20 August 2018

Orientador: Maria Luiza Silveira Mello / Dissertação (mestrado) - Universidade Estadual de Campinas, Instituto de Biologia / Made available in DSpace on 2018-08-20T03:24:19Z (GMT). No. of bitstreams: 1 Alvarenga_EleniceMonte_M.pdf: 2829254 bytes, checksum: 964b17aaf1c7f50d4471a7be569aaa6d (MD5) Previous issue date: 2011 / Resumo: A cromatina pode existir em núcleos interfásicos em dois estados distintos: como eucromatina e como heterocromatina, podendo ser esta constitutiva ou facultativa. Em células somáticas do final da fase ninfal dos hemípteros reduviídeos Triatoma infestans e Panstrongylus megistus há núcleos grandes, poliploides, nos quais a heterocromatina apresenta-se como corpos conspícuos (cromocentros), daí tais células apresentarem-se como um bom modelo para investigação de características morfológicas e funcionais da cromatina. Em estudos sobre a constituição cromatínica, a composição em bases do DNA é algo muito explorado, dado o conteúdo informativo dos achados. Já quando se objetiva a investigação da funcionalidade da cromatina, mais recentemente, tem-se feito uso da abordagem epigenética. Neste trabalho buscou-se investigar a composição em bases do DNA destas células, associando-a aos domínios cromatínicos aí existentes e também à presença das NORs. Por meio de colorações fluorescentes com Cromomicina A3 (CMA3)/Distamicina e 4',6-diamidino-2-fenilindol (DAPI)/Actinomicina D concluiuse que o DNA dos cromocentros de T. infestans e P. megistus são ricos em sequências AT e pobres em GC. Isto foi ainda confirmado por imunodetecção de 5-metilcitosina, que ocorreu somente na eucromatina, e tratamento de ninfas de T. infestans com 5-aza-2'-deoxicitidina (agente demetilante), seguido da análise dos fenótipos nucleares e análise de imagem, em que se observou expansão somente da área eucromática. Com o método de AgNOR evidenciou-se que a região rica em bases GC ao redor do cromocentro coincide com um acúmulo de proteínas argirofílicas, o que sugere associação com NORs. A presença de modificações epigenéticas nas caudas das histonas na cromatina destes insetos foi investigada por meio do uso de anticorpos contra marcadores epigenéticos específicos, permitindo identificar a participação diferencial dos mesmos na composição e na estrutura dos territórios heterocromáticos. Assim, observou-se hipoacetilação e hipermetilação de histonas na região do corpo heterocromático, o que indicaria uma possível ação da modificação de histonas na manutenção da estrutura heterocromática nas células somáticas de ambas as espécies de reduviídeos. Por meio da avaliação da ação de drogas inibidoras de deacetilases de histonas sobre a cromatina dos insetos percebeu-se que, quando ninfas de T. infestans e P. megistus foram tratadas com as drogas, houve aumento na frequência de necroses e, no caso específico do tratamento com tricostatina A (TSA) e butirato de sódio (NaBt), ocorreu descompactação da heterocromatina. Sugere-se que o tratamento com TSA e NaBt afete o processo de deacetilação de histonas, o qual seria, então, um fator importante na estruturação dos cromocentros. A observação da ocorrência de mudas e da sobrevivência de ninfas de T. infestans, realizada a fim de se avaliar a ação do ácido valproico (VPA) sobre o desenvolvimento dos insetos, mostrou que a droga, assim como a injeção de solução salina, reduziu seu período de sobrevivência, além de afetar a ocorrência de mudas / Abstract: Chromatin in interphase cell nuclei can be present in two distinct states: euchromatin and heterochromatin, which may be constitutive or facultative. In somatic cells at the end of the nymphal stage of Triatoma infestans and Panstrongylus megistus there are large nuclei, in which heterochromatin is presented as conspicuous bodies (chromocenters). These cells are an appropriate model for investigation of morphological and functional characteristics of the chromatin. In studies about chromatin constitution, the base DNA composition is explored due to the informational content of the findings. If the objective is to investigate the chromatin functionality, recently has been used the epigenetic approach. In the current study, the aim was to investigate the DNA base composition in these cells, associating with the chromatin domains therein and also the presence of NORs. Through fluorescent stains with Chromomycin A3 (CMA3)/Distamycin and 4',6-diamidino-2-fenilindole (DAPI)/Actinomycin D was found that the chromocenters DNA of T. infestans and P. megistus were AT-rich and GC-poor. This was also confirmed by immunodetection of 5-methylcytidine, which occurred only in the euchromatin, and by T. infestans nymphs treatment with 5-aza-2'- deoxycytidine (demethylating agent), followed by nuclear phenotypes analysis and image analysis, in which expansion was observed only in the euchromatic area. AgNOR test evidenced that the GC-rich region around the chromocenter coincides with an accumulation of argyrophilic proteins, suggesting association with NORs. Epigenetic modifications on histone tails in chromatin of these insects were investigated by using antibodies against specific epigenetic markers, in order to identify their differential participation in the composition and structure of these heterochromatic regions. It was observed hypoacetylation and hypermethylation in heterochromatic body area, suggesting a possible action of histones modification in the maintenance of the heterochromatic structure in somatic cells of both species of reduviids. Through evaluation of histones deacetylases inhibitors action on the chromatin, it was observed that when T. infestans and P. megistus nymphs were treated with these drugs there was an increase in the frequencies of necrosis, and in the specific case of Trichostatin A (TSA) and sodium butyrate (NaBt), occurred heterochromatin decondensation. It is suggested that treatments with TSA and NaBt could affect the histones deacetilation process, which would be an important factor in chromocenters structuring. Observations of the molting occurrence and survival of T. infestans nymphs, carried out in order to evaluate the action of valproic acid (VPA) on the development of insects, showed that this drug, as well as injection of saline, reduced the survival period, besides affecting the molting occurrence / Mestrado / Biologia Celular / Mestre em Biologia Celular e Estrutural

Triatoma

Panstrongylus

Heterocromatina

Epigênese genética

Triatoma

Panstrongylus

AT rich sequence

GC rich sequence

Heterochromatin

Genetic epigenesis

Footprint Analysis of the Transcriptional Control of Glycogen Phosphorylase 2 in Dictyostelium Discoideum

Col, Bekir

07 January 1998

Glycogen phosphorylase 2 (gp-2) is a key enzyme during the development of Dictyostelium discoideum. The gp-2 enzyme breaks down glycogen into glucose monomers that are subsequently used to synthesize the terminal end products of cellular differentiation. This gene is an ideal candidate for studying the process of selective gene expression because its product figures so prominently in the development of this organism, implying a dependable control mechanism responsible for its developmentally regulated expression. I present in this thesis the identification of several putative cis-acting elements of gp-2 as revealed through footprint analysis. Due to the extreme AT-bias characteristic of Dictyostelium promoters, footprinting conditions required intensive optimization with respect to template, nonspecific competitor, source of protein extract and DNase I digestion. Using an endlabeled fragment containing seven repeated sequences (3 TA boxes [TAATTATA], 2 TAG boxes [TAAAAATGGT] and 2 C boxes [ACCCACT]), purified replication protein A and several developmental nuclear extracts were tested for DNA binding activity. Small footprints were observed on the TAG and C boxes of the promoter for both protein sources. However, using a more sensitive footprinting strategy involving multiple rounds of primer extension, larger footprints spanning the same promoter regions were detected. In both cases, the appearance of the footprints coincided with the documented transcriptional activity of the gene. It can be concluded from the data obtained that the TAG and C boxes are very likely cis-acting elements involved in the regulation of gp-2 expression. / Master of Science

cell differentiation

Dictyostelium discoideum

DNase I footprint analysis

transcription

gene expression

AT-rich

looping

large footprints

replication protein A