1.16 The Nucleoid
A defining characteristic of prokaryotes is that they do not possess a membrane‐bound nucleus. Instead, prokaryotes have a nucleoid, a body within the cytoplasm that contains the genetic material but lacks a surrounding membrane (Piekarski 1937). The nucleoid is composed of the chromosome and associated molecules including RNA polymerase, DNA polymerase, DNA‐binding proteins, and RNA molecules (Dorman 2014b; Macavin and Adhya 2012). In electron micrographs of thinly sectioned bacteria, the nucleoid can be seen as an amoeboid shape surrounded by the electron‐dense ribosomes within the cytoplasm (Kellenberger 1952; Robinow and Kellenberger 1994). Staining of the DNA with 4′, 6‐diamidino‐2‐phenylindole (DAPI) has confirmed the presence of a zone around the nucleoid in E. coli and B. subtilis where translation can take place (Mascarenhas et al. 2001). While even more sophisticated imaging has improved our knowledge of the structure of the nucleoid, it has taken a multi‐pronged approach using a variety of techniques over several decades to bring about our current (but still incomplete) understanding of the bacterial nucleoid.
The chromosome is packaged within the bacterial cell in a conformation that permits gene expression and DNA replication to proceed. The 4.6 Mb circular chromosome of E. coli strain MG1655 has a circumference of 1.5 mm and, if opened out fully, a diameter of approximately 0.5 mm. In contrast, the bacterial cell is approximately 2 μm in length, 1 μm in diameter and has a volume of 1 fl, or 1 × 10−15 l (Dorman 2013; Kubitschek and Friske 1986). Understanding how the need to package the DNA efficiently is reconciled with the requirements of DNA replication, gene transcription, DNA recombination, and DNA repair is a major goal of research into the structure of the nucleoid.
1.17 The Chromosome Has Looped Domains
Examination of electron micrographs of thinly sectioned E. coli cells gives few clues as to the fine detail of chromosome organisation in the nucleoid. The images of chromosomes extruded from gently lysed E. coli obtained by Cairns (1963a,b) using autoradiography hint at a subdivision of the chromosome into looped, supercoiled domains. The nature of the domain boundaries was obscure but seemed to be associated with RNA (Kavenoff and Bowen 1976). Analysis with electron microscopy suggested that the chromosome was subdivided into between 12 and 80 supercoiled loops (Delius and Worcel 1974).
Sinden and Pettijohn (1981) used photobinding of trimethylpsoralen to intracellular DNA to estimate the number of independently looped domains. This agent binds to duplex DNA at a rate that is proportional to the superhelical tension in the DNA (Sinden et al. 1980). By estimating the number of gamma‐radiation‐induced nicks that were required to release most of the superhelical tension, an estimate of the number of topologically independent domains was obtained. For E. coli growing with a generation time of 30 minutes, it was estimated that the chromosome is divided into between 33 and 53 independent domains (or between 90 and 150 domains per nucleoid) (Sinden and Pettijohn 1981). The existence of independent domains is an important concept in nucleoid architecture: genes in one domain may be isolated from DNA topological changes taking place in other domains, making gene location along the chromosome significant for reasons other than differences in copy number arising as a result of gene distance from oriC.
More refined measurements of domain number in the E. coli chromosome or that of its close relative, Salmonella enterica serovar Typhimurium, have been made by exploiting site‐specific recombination reactions that can take place within but not between domains, by counting the number of looped domains in multiple images of extruded chromosomes, and by releasing superhelical tension from domains using restriction enzymes and observing the distance over which an effect on the transcription of a supercoiling‐sensitive gene can be exerted (Postow et al. 2004; Stein et al. 2005). The results from these experimental approaches indicate that the chromosome is subdivided into about 400 independent domains in E. coli cells during exponential growth, with each being approximately 12–14 kb in length. The boundaries between the domains do not seem to be fixed and fewer of them are found in bacteria that have entered stationary phase (Staczek and Higgins 1998).
1.18 The Macrodomain Structure of the Chromosome
The bacteriophage lambda integrase‐mediated site‐specific recombination system has been exploited in studies of nucleoid organisation in E. coli and Salmonella (Garcia‐Russell et al. 2004; Valens et al. 2004). Recombination between copies of the lambda attachment site requires physical contact between the sites and these can be created by random collision (Crisona et al. 1999; Dorman and Bogue 2016). Sites placed at different distances from one another around the chromosome can be assessed for interaction frequency, providing an estimate of the frequency of contact between different parts of the chromosome. At the same time, regions of the chromosome that rarely interact have also been discovered. This analysis led to the proposal that the chromosome is divided into a small number of large territories called macrodomains (Valens et al. 2004) (Figure 1.1). E. coli and its close relatives have four macrodomains (Ori, Left, Ter, and Right) and two non‐structured (NS) regions: NS‐Left and NS‐Right (Cameron et al. 2017; Jiang et al. 2015; Thiel et al. 2012). The NS domains are determined by their proximity to the Ori macrodomain: any region that is placed next to Ori acquires the features of an NS domain (Duigou and Boccard 2017).
1.19 The Chromosome Displays Spatial Arrangement Within the Cell
The bacterial chromosome is oriented in the cytoplasm with reference to the poles and the midpoint of the cell (Figure 1.9). This positioning is important for the successful segregation of the daughter chromosomes at cell division and it assigns domains to specific regions of the cytoplasm. Experiments using fluorescence in situ hybridisation (FISH) in E. coli show that in newborn cells, Ori and Ter are located at the cell poles and that genetic loci in between follow approximately the gene order along the chromosome (Niki et al. 2000). Before the initiation of chromosome replication, Ori and Ter move to the mid‐cell position. Chromosomes with gross rearrangements of the macrodomains misplace Ori and Ter, leading to the appearance of anucleate daughter cells at cell division (Niki et al. 2000).
FISH experiments involve the permeabilisation and fixing of the bacterial cells; these treatments may produce artefacts, making less intrusive approaches more desirable. Experiments in which arrays of binding sites for fluorescently labelled DNA‐binding proteins are placed at specific chromosomal locations have allowed chromosome dynamics to be studied in live bacteria (Robinett et al. 1996). This approach has revealed that in slow‐growing E. coli cells, the origin and terminus are found at mid‐cell and the replichores are located in each cell half (Nielson et al. 2006b; Wang et al. 2006) (Figure 1.9). In fast‐growing E. coli cells, the Ori copies are found at the cell poles while the Ter region is recovered from the pole to the mid‐cell position as the replication forks close in (Youngren et al. 2014) (Figure 1.9). This situation is reminiscent of that described in B. subtilis for the Ori and Ter regions during chromosome replication (Teleman et al. 1998; Webb et al. 1997). C. crescentus has also served as an important model organism in nucleoid structure studies and its chromosome has been observed as adopting an arrangement in which Ori is located at one cell pole and Ter at the other (Viollier et al. 2004) (