| dc.description.abstract | Cerebral small vessel disease (SVD) is a vascular neurodegenerative disease which is
the leading cause of vascular dementia and causes 20% of strokes. 20-30% of those
over 80 show signs of the disease as white matter hyperintensities on MRI scans,
doubling their risk of stroke and trebling their risk of dementia. Sporadic SVD is
thought to be caused by hypertension but 30% of sufferers are normotensive and an
alternative hypothesis implicates loss of integrity of the blood brain barrier (BBB).
To investigate this, I studied brains from normotensive people with early stage SVD
and found reduced capillary endothelial claudin-5 (a BBB tight junction protein), more
oligodendrocyte precursor cells (OPCs; the precursors to myelinating
oligodendrocytes), and more microglia/macrophages compared to controls.
Furthermore, in a relevant rat model of spontaneous SVD, the Stroke Prone
Spontaneously Hypertensive Rat (SHRSP; disease model; DM) I found that reduced
endothelial claudin-5 was the earliest change, appearing at 3 weeks of age, followed
by OPC proliferation, appearing at 4 weeks, and then increased number of
microglia/macrophages, appearing at 5 weeks. Importantly, all these changes occurred
at a young age (< 5 weeks), before any measurable hypertension. These changes were
confirmed in an ex vivo slice culture model (i.e. removing blood flow), ruling out direct
damage by leakage of blood components through an impaired BBB and suggesting an
inherent endothelial cell dysfunction as the primary cause, with secondary BBB
defects.
This hypothesis of endothelial dysfunction is supported by increased endothelial cell
proliferation in both human SVD tissue and the DM rats, and lower levels of
endothelial nitric oxide synthase (eNOS) in brains of DM rats. To study this further I
isolated primary brain microvascular endothelial cells (BMECs) from DM and control
rats and found that those from DM rats formed less mature tight junctions (less
membranous claudin-5) than control BMECs. I also found that conditioned media
(CM) from DM BMECs causes OPCs in culture to proliferate more and mature less.
This indicates that the endothelial dysfunction is inherent to the endothelial cells,
rather than induced by other cell types, and through secreted factors causes OPC
changes mirroring what is seen in vivo. Using an antibody array, I identified HSP90α
as a candidate secreted factor and showed that it is necessary (by blocking the protein
in CM) and sufficient (by adding recombinant HSP90α) to induce the maturation
phenotype in OPCs, but not the proliferation phenotype.
The idea that endothelial dysfunction causes SVD begs the question of what causes
endothelial dysfunction, especially in our inbred DM rat strain. To establish this, I
reanalysed sequencing data of the DM and control rats from a previously published
study, searching for mutations which lead to truncated proteins in genes expressed in
brain endothelial cells. We confirmed the candidate gene Atp11b, a phospholipid
flippase, was mutated as predicted. I found that knocking down Atp11b using siRNA
in a control endothelial cell line caused endothelial dysfunction and a loss of tight
junction maturity, and that CM from these cells causes OPCs to proliferate more and
mature less, mirroring what we see in primary DM BMECs and suggesting that Atp11b
has a key function in promoting normal endothelial function. Furthermore, I showed
that knocking down Atp11b causes cells to secrete increased levels of HSP90α. I
propose a mechanism whereby ATP11B regulates the retention of HSP90α within
endothelial cells, which in turns regulates eNOS levels and activity, as has been shown
previously.
In summary, this work shows that there are many pre-symptomatic changes which
occur in the brain in the development of SVD in DM rats, and that these are ultimately
caused by endothelial dysfunction. As these changes are similar to those found in
spontaneous human SVD, I propose that endothelial dysfunction is a key mechanism
of human SVD, which may in the future lead to new therapies. | en |
