Quantification of myelin loss in frontal lobe white matter in vascular dementia, Alzheimer’s disease, and dementia with Lewy bodies

Table 1 provides the demographics and the pathological features of the subjects. All the patients were prospectively assessed in Newcastle and the duration of clinical disease ranged between 6 and 12 years. We obtained coronal blocks of tissue from the frontal and temporal lobes from the Newcastle Brain Tissue Resource (NBTR) and excluded cases with pathological diagnoses of co-existing VaD and AD or VaD and DLB. Thus, 82 cases were included in this study to select cases for relatively single processes, which consisted of 12 controls, 31 DLB cases, 19 AD cases, and 20 VaD cases. Autopsies were performed within 12–36 h after death. The post-mortem intervals between death and tissue retrieval were not different between the groups. There were also no differences in the length of fixation of tissue in formalin between the cases and controls^. Brains were fixed for 4–6 weeks. As previously described [30], the neuropathological diagnoses of VaD [28], AD [9, 37], and DLB [35] were made by thorough histopathological examination of extensively sampled brain sections. The clinical study had ethical approval from the local Newcastle Ethics committees and all participants gave written consent to brain tissue donation. Use of brain tissue was also approved by the local research ethics committee of the Newcastle upon Tyne Hospitals NHS Foundation Trust and the NBTR committee.

Ten and 20-μm thick paraffin-embedded tissue sections were cut from the frontal lobe at the level of the olfactory bulbs and the temporal lobe at the level of the anterior hippocampus and stained for H&E and LFB (20 μm) and for immunohistochemistry (10 μm). To minimize variability in LFB staining and immunohistochemical intensity, control sections were included, tissue sections were prepared by the same technician and stained with or using freshly prepared tinctorial and buffer solutions.

Myelin density was determined in a large series of LFB-stained serial coronal sections from cases and controls to select representative regions of interest (ROI) for analyses. The analyses were performed essentially as previously described [51]. To determine the myelin index, the WM was outlined automatically using the wand tool. When the border between the neocortex and the WM was obscured due to severe myelin loss, the WM was outlined manually using the semiautomatic trace tool instead of the wand tool. Any incidental border region of the cortex mixed in the outlined WM area was excluded from the analysis (Fig. 1, asterisk). The detected range of grey levels within the WM, corresponding to the staining intensity, from the point 0–127 (0, white; 255, black) was divided into four quartiles (the first quartile 0–29, the second 30–62, the third 63–94, and the fourth 95–127). The percent area (%area) for each quartile was calculated. The median grey level of each quartile (14.5, 46.0, 78.5, and 111.0), an estimate for the staining intensity, was then multiplied by %area/100 in each quartile, which gave the total myelin index [51]. Braak staging [8] and plaque burden scores were used to explore the relationship with the myelin index. Chi-square analysis was performed to determine if higher Braak stage (≥IV) affected myelin index (cut-off score = median value of myelin index, 44.0 for the frontal lobe; 40.0 for the temporal lobe) or amyloid score (none/sparse or moderate/severe) in the combined cases of AD and DLB (28 cases with Braak stage 0 through III and 22 cases with Braak stage IV through VI). The H&E-stained slides were examined in parallel but independently of the findings in the LFB images or case diagnosis. The WM damage was categorized as one of the following four grades as previously described [43] and corroborated by quantitative biochemical data [14]: (1) normal, normal WM; (2) mild, no appreciable reduction in axonal meshwork density and easily recognized long axons with occasional axonal debris and a slightly increased number of reactive astrocytes; (3) moderate, a slight reduction of axonal meshwork density and a reduction of oligodendroglial cell nuclei and a further increased number of reactive astrocytes; and (4) severe, a marked reduction of myelin, axons and oligodendroglial cell nuclei with relatively marked astrocytic reaction and loosely scattered macrophages, but no complete cerebral infarct. When several grades were observed in one section, the dominant grade represented the section.

Frontal sections from 59 cases (controls n = 8, DLB n = 18, AD n = 14, VaD n = 19) with WM area > 15 mm² were stained with rabbit anti-dMBP sera (AB5864, Millipore, Billerica, MA, USA) essentially as previously described [51] using the Vectastain ABC System [27]. Images of 15–22 randomly selected ROIs in the WM were captured and then analysed [51]. The percentage immunostained area was measured within each field, which was averaged to yield %dMBP for all the sections. Infarcted areas were always excluded from the analysis because of the entirely different patterns of dMBP staining. All of the above analyses were performed blind to the diagnosis by labelling the sections with arbitrary numbers.

Serial sections from five cases of VaD and AD each and three cases of DLB immediately adjacent to those stained for dMBP were stained with an antibody against GSTpi (Thermo Fisher Scientific Anatomical Pathology, Cheshire, UK) to determine the density (number of oligodendrocytes/mm²) and the mean size (μm²) of oligodendrocytes. For such staining, 15–22 images of the ROI as for dMBP staining were similarly captured and analysed using computer-assisted analysis. Our preliminary data suggested that staining quality exponentially diminished with prolonged postmortem delay, especially when it exceeded 30 h. Some of the sections showed high background and reduced contrast, making it difficult to correctly identify oligodendrocytes. However, all cells with stained area of 4.2–25.3 μm² (40–240 pixels) were counted after testing for accuracy for oligodendrocyte size rather than macrophages or other cells. Non-specific reactivities such as in blood vessel walls, mostly linear in shape with major axis larger than 24 pixels and minor axis smaller than 6 pixels, and macrophages were distinguished from the oligodendrocytic staining and automatically excluded from the analysis. In addition to GSTpi, we tested with success a range of other antibodies to detect mature oligodendrocytes including those to 2′,3′-cyclic nucleotide 3′-phosphodiesterase (clone 11-5b, Sigma-Aldrich, St. Louis, MO, USA), myelin oligodendrocyte glycoprotein (courtesy of Prof Richard Reynolds, Imperial College), Nogo-A (Abcam, Cambridge, UK), OLIG2 (Abcam) and SRY-box containing gene 10, SOX10 (clone 20B7, R&D Systems, Abingdon, UK).

Statistical analysis was performed using StatView5.0 (SAS Institute, Cary, NC, USA). Frontal and temporal myelin densities were analysed separately. The %area for the first or second quartile, the myelin index, and %dMBP were compared among the four groups by an unpaired t test. Frontal and temporal WM were analysed separately for the %area and myelin index. Pearson correlation analysis was performed to observe possible correlation of %dMBP with the %area for the first or second quartile, with myelin index, or with the size/density of oligodendrocytes. Chi-square analysis was performed to determine any correlation of myelin index with the Braak stage or plaque density in the AD and DLB cases combined (all except one DLB case showed Braak stage ≥ I). A two-level regression model was also applied to the hierarchical data set, with size or density of oligodendrocytes as a single outcome and %dMBP as a response variable that was measured at the ROI (lower) level, and with age, gender, disease (disease code; 0 = AD and 1 = VaD), and mean %dMBP as explanatory variables at the case (higher) level using the HLM6 software. For all analyses, the level of statistical significance was set at P < 0.05.