. Shown is a single optical section made with a
confocal microscope. Bottom: Same nucleus stained with
DAPI and recorded with a
CCD camera. The Barr body is indicated by the arrow, it identifies the inactive X (Xi). At present, very little is known about either the mechanisms orchestrating the timing program or its biological significance. However, it is an intriguing cellular mechanism with links to many poorly understood features of the folding of chromosomes inside the cell nucleus. All eukaryotes have a timing program, and this program is similar in related species. This indicates that it is either important itself, or something important influences the program. It is unlikely that replicating DNA in a specific temporal order is necessary simply for the basic purpose of duplicating a DNA molecule. More than likely, it is related to some other chromosomal property or function. Replication timing is correlated with the expression of genes such that the genetic information being utilized in a cell is generally replicated earlier than the information that is not being used. We also know that the replication-timing program changes during development, along with changes in the expression of genes. For many decades now, it has been known that replication timing is correlated with the structure of chromosomes. For example,
female mammals have two X chromosomes. One of these is genetically active, while the other is inactivated early in development. In 1960, J. H. Taylor showed that the active and inactive X chromosomes replicate in a different pattern, with the active X replicating earlier than the inactive X, whereas all the other pairs of chromosomes replicate in the same temporal pattern. It was also noticed by
Mary Lyon that the inactive X took on a condensed structure in the nucleus called the
Barr body (
Figure 5) at the same time during development as the genetic inactivation of the chromosome. This may not come as too much of a surprise, since the packaging of DNA with proteins and RNA into
chromatin takes place immediately after the DNA is synthesized. Therefore, replication timing dictates the time of assembly of chromatin. Less intuitive is the relationship between replication timing and the three-dimensional positioning of chromatin in the nucleus. It is now well-accepted that chromatin is not randomly organized in the cell nucleus, but the positions of each chromosome domain relative to its neighboring domains is characteristic of different cell types, and after this geography is established in each newly formed cell, the chromosome domains do not move appreciably until the next cell division. In all multi-cellular organisms where it has been measured, early replication takes place in the interior of the nucleus and the chromatin around the periphery is replicated later. Recently developed methods to measure the points where different parts of chromosomes touch each other are almost perfectly aligned to when they replicate. One possibility is that these different compartments within the nucleus, established and maintained without the aid of membranes or physical barriers, set thresholds for the initiation of replication so that the more accessible regions are the first to replicate. Another possibility is that the replication timing of a section of DNA contributes to the packaging of that DNA. It has been demonstrated that the protein
Rif1 is involved in regulating this process. ==Replication timing and disease==