Standard protocol approvals, registrations, and patient consents

All patients included in the Irish ALS register between January 1, 1994, and December 31, 2016, were invited to participate in the study. Informed written consent for the study was obtained from all participants. This study was approved by the Beaumont Hospital Research Ethics Committee (15/40).

Diagnostic criteria for FALS

The presence and classification of FALS was determined using our previously defined criteria (figure 1).¹⁷

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Figure 1

Byrne criteria for familial amyotrophic lateral sclerosis (FALS)

Analysis of register data

Data from the Irish ALS register from 1994 to 2016 were interrogated. All cases reporting a history of suspected or confirmed ALS or FTD in at least 1 relative were collated. Where necessary, genealogical records were reviewed. The DNA database was cross-referenced with the clinical database, and the genetic status was determined in all cases for whom DNA was available. Additional individuals with a known gene variant, not previously identified by a family history of ALS or FTD, were collated. Cases with a diagnosis of Kennedy disease were excluded. Individuals who had a family history suspicious for ALS (e.g., relative died of “muscle wasting disease”), in whom we could not confirm the diagnosis, were excluded. Similarly, individuals with a relative with dementia, in whom the nature of the dementia could not be accurately determined, were excluded.

Our previously reported criteria were applied to all identified FALS cases. Annual age-standardized incidence rates for FALS and FALS subclassifications were calculated as a proportion of the total number of ALS cases diagnosed annually, using the pooled Irish ALS register population from 1994 to 2016 and considering the following age bands: ≤39, 40–49, 50–59, 60–69, 70–79 and 80+ years.

Where multiple members of the same kindred were identified, pedigrees were constructed to include first-, second-, and third-degree relatives where possible. All newly diagnosed individuals from previously identified kindreds were identified. Crude incidence rates of newly diagnosed individuals from known families were calculated as a proportion of total number of ALS families presenting annually. Dates of diagnosis of FALS for all cases were obtained from the ALS register and cross-referenced against medical records where applicable. All cases were grouped by whether they were recategorized from SALS to FALS or identified as FALS at the time of diagnosis. Annual rates of recategorization were calculated by dividing the number of recategorized FALS individuals by the number of individuals diagnosed with ALS annually.

Analysis by additional phenotype and endophenotype

All cases with a confirmed family history of FTD were identified. Secondary analysis identified all probands with a confirmed family history of all-type dementia and/or schizophrenia/psychosis. The crude incidence rates of probands with a confirmed family history of FTD, all-type dementia, and possible familial endophenotypes (e.g., schizophrenia/psychosis¹³) were calculated by dividing by the number of patients diagnosed with ALS annually.

Genetic screening and analysis

All patients were tested for established high-penetrance ALS-associated variants. Patients were screened for the presence of the pathogenic GGGGCC hexanucleotide repeat expansion in C9orf72 by repeat-primed PCR as described previously.¹⁸ This methodology has previously been validated with positive and negative controls using reverse transcriptase PCR and Southern blots. Amplified fragments were measured by capillary electrophoresis on an Applied Biosystems 3500 Series Genetic Analyzer and visualized using Gene Mapper v.4.0. Patients with 30 hexanucleotide repeats or above were deemed positive for the expansion. Next-generation DNA sequencing was performed through Illumina paired-end, PCR-free, whole-genome sequencing and Illumina paired-end, target-enriched sequencing. Sequence data were generated for 676 patients and 446 population-matched controls. Participants were screened for exonic and splice-site variants in the exons of 30 genes considered to be linked to ALS (ALS2, ANG, CHCHD10, CHMP2B, DAO, DCTN1, ELP3, ERBB4, FIG4, FUS, hnRNPA1, LMNB1, MATR3, NEFH, OPTN, PFN1, PRPH, SETX, SIGMAR1, SOD1, SPAST, SPG11, SQSTM1, TAF15, TARDBP, TBK1, UBQLN2, UNC13A, VAPB, and VCP). To screen for high penetrance, variants that were present in any controls or at a maximum allele frequency exceeding 0.05 in reference population data sets were filtered. Variants that were present in the ALSonline genetics database (ALSoD)¹⁹ or the Human Gene Mutation Database V.2017.2²⁰ and are reported in the literature as being familial or highly penetrant were considered to be mendelian causes of ALS. Patients for whom DNA was not available and without confirmed family history of ALS or FTD were categorized as nonfamilial cases. All cases with an established mendelian-inherited ALS gene variant were identified, and the crude incidence rate of mendelian-inherited ALS was calculated by dividing by the number of patients diagnosed with ALS annually.

Incidence of FALS

The mean annual crude FALS incidence rate was 11.1% (95% confidence interval [CI], 8.9–13.3) for the study period, and the corresponding mean age-standardized FALS incidence rate was 11.1% (95% CI, 8.8–13.4). However, the age-standardized FALS incidence rate increased steadily from 5.2% in 1994 to 19.1% in 2016, representing an overall increase of 0.7% (95% CI, 0.5–0.9, p < 0.0001) per annum (figure 3A). Using our previously published criteria for “definite FALS,” the mean age-standardized incidence rate was 4% (95% CI, 2.9–5.0) for the entire study period. However, between 1994 and 2016, this increased at a rate of 0.2% (95% CI, 0.01–0.3, p = 0.007) annually (figure 3B). For “probable FALS,” the age-standardized incidence rate was 3.1% (95% CI, 2.3–3.9) but did not increase with time (p = 0.318) (figure 3C). Conversely, the age-standardized incidence for “possible FALS” increased by 0.4% (95% CI, 0.2–0.5, p < 0.0001) annually, with an overall mean rate of 4.6% (95% CI, 3.1–6.1) (figure 3D). There was no difference between the total FALS (b = 0.007) and combined “definite” and “probable FALS” (b = 0.003) beta coefficients (p = 0.671) (figure 3E).

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Figure 3

Temporal trends in FALS incidence

Temporal trends in age-standardized FALS incidence for total FALS (A), definite FALS (B), probable ALS (C), and possible FALS (D). Temporal trends in age-standardized FALS incidence for total FALS compared with definite and probable FALS (E). ALS = amyotrophic lateral sclerosis; FALS = familial ALS.

FALS from previously identified families and recategorized FALS

A mean of 2.9% (95% CI, 1.8–4.1) of individuals diagnosed with ALS each year were from known FALS families, increasing by 0.3% annually (95% CI, 0.2–0.4, p < 0.0001). The relative contribution of newly diagnosed individuals from known families increased annually (p = 0.001), accounting for 50% of all FALS diagnoses in 2016. To prevent an underestimation of effect size due to unrecognized FALS in SALS individuals (i.e., those in whom a second family member has not yet been affected), the final 3 years of data collection were excluded. For the remaining years, the overall mean rate of recategorization from sporadic to FALS was 3% (95% CI, 2.6–3.8) annually. This did not change with time (p = 0.177).

Mendelian-inherited ALS

From 1999 to 2016, the mean crude incidence rate for known mendelian-inherited ALS was 4.49% (95% CI, 2.8–6.2) annually. A temporal increase of 0.4% (95% CI, 0.2–0.6) annually (p = 0.02) was observed, driven by C9orf72-positive ALS patients, who accounted for 89 of 94 known mendelian-inherited forms. The other cases, all of which were sporadic, were associated with mutations in TARDBP (1), FUS (2), SQSTM1 (1), and a previously recognized rare SOD1 variant.