To the editor:
Partial albinism and primary immunodeficiency occur in several autosomal recessive disorders, including Hermansky-Pudlak syndrome type 2 (HPS2, Online Mendelian Inheritance in Man [MIM] #608233), Chediak-Higashi syndrome (MIM#214500), Griscelli syndrome types 1 (MIM#214450) and 2 (MIM#607624), and endosomal-adaptor protein p14 deficiency (MIM#610798).1-6 At least 15 recessive mouse mutations have been described that also are characterized by partial albinism and immunodeficiency and/or bleeding disorders and that appear to be homologous to the human diseases.7-10
A 17-year-old, northern Italian female with oculocutaneous albinism, nystagmus, and normal neurologic development presented with recurrent cutaneous infections but without hemorrhagic episodes. At 6 years of age, she had a prolonged episode of fever with convulsions. At presentation, she had thrombocytopenia (111 000 platelets/μL) and leucopenia (2600 leucocytes/μL, 2300 neutrophils/μL; 300 lymphocytes/μL). Platelet aggregation tests were normal.
Nucleotides (37.7 million) of exons (the exome) were enriched 44-fold from genomic DNA from the patient and sequenced to an average, uniquely aligned coverage of 135-fold.11 No mutations were identified in known immunodeficiency disease genes. Only one novel variant had high likelihood of pathogenicity and was unique to the patient among ∼ 250 Children's Mercy Hospital exomes and the NHLBI exome collection (http://evs.gs.washington.edu/EVS/). It was a homozygous nonsense mutation, c.232C > T (p.Q78X), in exon 3 of pallidin (PLDN, chr15:45895305C > T, relative to human genome build 37, supplemental Figure 1A [available on the Blood Web site; see the Supplemental Materials link at the top of the online article]), present in all 65 aligning sequences. This mutation was confirmed to be homozygous in the patient and heterozygous in her parents by Sanger sequencing (supplemental Figure 1B), and was associated with absent PLDN protein expression (supplemental Figure 1C).
Because intracellular trafficking and degranulation of specialized lysosomes are impaired in HPS2,2,3,5 we sought such defects in the patient. The proportion of resting and IL-2–activated NK cells expressing the lysosomal membrane protein CD107a on the surface was increased (6% and 14% of NK cells from the patient, respectively, versus 0.6% and 2% in healthy controls, respectively, Figure 1A). However, these increases were not as marked as in HPS2 (24% in IL-2–activated NK cells [S.P., G.T., R.B., unpublished observations] but at odds with one case report4,5 ). PLDN replacement in NK cells from the patient decreased CD107a expression to normal (Figure 1B).
NK cells from the patient had intermediate cell-surface expression of CD63, another lysosomal membrane protein altered in HPS21,4,6 (17% in patient, 9% in controls, and 28% in an HPS2 patient, Figure 1A). Degranulation, as measured by change in surface expression of CD107a on IL-2–activated NK cells after challenge with LCL 721.221 target cells, was less than controls (Figure 1C).
Cytolytic activity of resting and IL-2–activated NK cells from the patient was reduced (Figure 1C). Low NK activity did not correlate with reduced expression of activating receptors,12 as assessed by NKp30, NKp46, NKG2D, and CD244 (2B4) levels on NK cells cultured with IL-2 for 3 weeks.
Pallid mice have reductions in coat and eye pigmentation, lysosomal enzyme secretion, chemotactic release of neutrophil elastase, and neutrophil killing of Leishmania, together with prolonged bleeding because of storage pool deficiency.7-10 Here, we have shown that a homozygous nonsense mutation in the homologous human gene was associated with partial oculocutaneous albinism, leucopenia, and recurrent infections. While in preparation for publication, a patient with partial albinism and absence of platelet δ granules was reported to have the same mutation in PLDN.13 That patient did not have recurrent infections. We have also shown the PLDN mutation to be associated with defective NK-cell degranulation and cytolysis, and with abnormal lysosomal markers on NK cells that were similar to, but distinct from, those in HPS2. Some of these were corrected by PLDN replacement. The symbol HPS9 has been approved for PLDN-associated disease.
Authorship
The online version of this article contains a data supplement.
Acknowledgments: The authors thank Alessandro Moretta for providing NK receptors anitbodies. This work was funded by grants from National Institutes of Health (AI066569 and DK091823) and the Marion Merrell Dow Foundation to S.F.K., PRIN2009 and EU Grant FP7 (HLH-cure) to R.B., and by in-kind support from Illumina Inc and British Airways PLC. A deo lumen, ab amicis auxilium.
Contribution: R.B. obtained the clinical information, led the functional studies and wrote the manuscript; S.C. and F.C. performed Sanger sequencing and immunoblotting studies; M.E.C. and A.P. were following the child; A.P. has performed PLDN sequence analysis in control subjects and immunoblotting experiments; M.G. has performed flow cytometry and neutrophil studies; G.T. and S.P. have performed NK cell studies; C.J.B. contributed computer programming and data analysis; D.L.D. made the sequencing libraries, performed target enrichments and data analysis; A.P. performed the transfection studies; N.A.M. carried out data pipelining, software development and bioinformatics; S.L.H. carried out literature research and data analysis; L.Z. and G.P.S. performed sequencing; and S.F.K. wrote the manuscript and carried out data analysis.
Conflict-of-interest disclosure: L.Z. and G.P.S. were employees of Illumina Inc at the time the research was performed. The remaining authors declare no competing financial interests.
The PLDN mutation was deposited at the NCBI ClinVar.
Correspondence: Dr Raffaele Badolato, Universita di Brescia, c/o Spedali Civili, Brescia, BS 25123, Italy; e-mail: badolato@med.unibs.it.
References
National Institutes of Health