Mannose-Binding Lectin Levels in Critically Ill Children With Severe Infections*

Madsen, Erik; Levy, Emily R.; Madden, Kate; Agan, Anna A.; Sullivan, Ryan M.; Randolph, Adrienne G.

doi:10.1097/pcc.0000000000001000

Cited by 5 publications

(4 citation statements)

References 55 publications

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“…A large cohort of hospitalized children with meningococcemia also did not have higher carriage of O alleles (49). In single center nested case-control PICU studies, we reported no differences in carriage of low-producing MBL2 variants in patients with severe infections (22) but others reported a 2-fold overall increase in carriage of the O allele with an increase in homozygotes (50). Although MBL2 haplotypes associated with deficiency appear to be a risk factor for a range of infections in neonates or other immune compromised patients, our study adds to the literature that carriage of low-producing MBL2 variants does not increase risk of severe viral infections (51).…”

Section: Discussionmentioning

confidence: 66%

“…MBL deficiency is common, and may occur in 30% of the population depending on what MBL level cutoff is used for defining it; deficiency has been defined variably as <1,000, <500, <200, or <100 ng/mL (21). In critically ill patients, serum levels may be influenced by inflammation, diluted by fluid resuscitation, or raised via fresh frozen plasma transfusion, so genotype has been used as an inexact proxy to estimate pre-illness MBL deficiency (17, 22).…”

Section: Introductionmentioning

confidence: 99%

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Evaluation of Mannose Binding Lectin Gene Variants in Pediatric Influenza Virus-Related Critical Illness

Levy

Yip²,

Super

et al. 2019

Front. Immunol.

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Background: Mannose-binding lectin (MBL) is an innate immune protein with strong biologic plausibility for protecting against influenza virus-related sepsis and bacterial co-infection. In an autopsy cohort of 105 influenza-infected young people, carriage of the deleterious MBL gene MBL2 _Gly54Asp(“B”) mutation was identified in 5 of 8 individuals that died from influenza-methicillin-resistant Staphylococcus aureus (MRSA) co-infection. We evaluated MBL2 variants known to influence MBL levels with pediatric influenza-related critical illness susceptibility and/or severity including with bacterial co-infections. Methods: We enrolled children and adolescents with laboratory-confirmed influenza infection across 38 pediatric intensive care units from November 2008 to June 2016. We sequenced MBL2 “low-producer” variants rs11003125(“H/L”), rs7096206(“Y/X”), rs1800450 Gly54Asp (“B”), rs1800451 Gly57Glu (“C”), rs5030737 Arg52Cys (“D”) in patients and biologic parents. We measured serum levels and compared complement activity in low-producing homozygotes (“B/B,” “C/C”) to HYA/HYA controls. We used a population control of 1,142 healthy children and also analyzed family trios (PBAT/HBAT) to evaluate disease susceptibility, and nested case-control analyses to evaluate severity. Results: We genotyped 420 patients with confirmed influenza-related sepsis: 159 (38%) had acute lung injury (ALI), 165 (39%) septic shock, and 30 (7%) died. Although bacterial co-infection was diagnosed in 133 patients (32%), only MRSA co-infection ( n = 33, 8% overall) was associated with death ( p < 0.0001), present in 11 of 30 children that died (37%). MBL2 variants predicted serum levels and complement activation as expected. We found no association between influenza-related critical illness susceptibility and MBL2 variants using family trios (633 biologic parents) or compared to population controls. MBL2 variants were not associated with admission illness severity, septic shock, ALI, or bacterial co-infection diagnosis. Carriage of low-MBL producing MBL2 variants was not a risk factor for mortality, but children that died did have higher carriage of one or more B alleles (OR 2.3; p = 0.007), including 7 of 11 with influenza MRSA-related death (vs. 2 of 22 survivors: OR 14.5, p = 0.0002). Conclusions: MBL2 variants that decrease MBL levels were not associated with susceptibility to pediatric influenza-related critical illness or with multiple measures of critical illness severity. We confirmed a prior report of higher B allele carriage in a relatively small number of young individuals with influenza-MRSA asso...

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Section: Discussionmentioning

confidence: 66%

Section: Introductionmentioning

confidence: 99%

Evaluation of Mannose Binding Lectin Gene Variants in Pediatric Influenza Virus-Related Critical Illness

Levy

Yip²,

Super

et al. 2019

Front. Immunol.

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“…However in a recent study, MBL levels had no association with infection status at admission, or with progression from systemic inflammatory response syndrome to sepsis or septic shock in children admitted with severe or life-threatening illness 16 . It has also been shown that MBL deficiency is not associated with a susceptibility to influenza-related critical illness in children 17 .…”

Section: Introductionmentioning

confidence: 81%

Respiratory outcomes at five-year follow-up in children with MBL deficiency: a cohort study

Ramphul

Poghosyan

Afzaal

et al. 2021

Preprint

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Introduction Mannose-binding lectin (MBL) serum protein, is an important molecule of the innate immune system that is involved in antimicrobial recognition and clearing responses. There is no conclusive evidence that MBL deficiency is associated with adverse respiratory consequences. Aim We explored whether there is a difference in clinical, radiological and microbiological characteristics in children with MBL deficiency presenting with troublesome respiratory symptoms (frequent, recurrent, persistent or very severe), as compared to those who are MBL-sufficient. Methods We performed a retrospective study looking at MBL measurements in children over a period of 10 years in a large teaching hospital, with a minimum follow-up period of 5 years from the time of the MBL measurement to the year 2019. Results 32% of children with MBL deficiency and 30% of those with MBL sufficiency had positive microbiology. 23% of children with MBL deficiency and 24% of those with MBL sufficiency had radiological changes on plain radiographs. 28% of children with MBL deficiency and 33% of those with MBL sufficiency had suboptimal vaccine responses to primary immunisations. 67% of the MBL-deficient children had suboptimal vaccine responses to booster immunisations, compared to 40% of the MBL-sufficient group. Conclusion We conclude that there is no difference at five year follow-up in clinical, radiological and microbiological characteristics between children who are MBL-deficient as compared to those who have sufficient levels. These results add to the existing body of literature that shows no statistically significant association between MBL deficiency and susceptibility to recurrent respiratory tract infection in children.

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“…Up to this day, a wide spectrum of other methods have been used for detection of MBL2 gene variants, including commercially available TaqMan assays [ 27 ], high-resolution melt analysis (HRMA) [ 28 ], reverse hybridization with membrane-immobilized sequence-specific oligonucleotide probes (reverse PCR-SSOP) [ 29 ], PCR with sequence-specific primers (SSP-PCR) [ 30 , 31 ], PCR and restriction-fragment length polymorphism (PCR-RFLP) analysis [ 32 ], an oligonucleotide ligation assay [ 33 , 34 ], a single-strand conformation polymorphism technique (PCR-SSCP) [ 35 ], the iPLEX assay on a MassArray system [ 36 ], Sanger sequencing [ 37 ], and pyrosequencing [ 38 ].…”

Section: Discussionmentioning

confidence: 99%

A SNaPshot Assay for Determination of the Mannose-Binding Lectin Gene Variants and an Algorithm for Calculation of Haplogenotype Combinations

Mrázková

Sistek²,

Lochman

et al. 2021

Diagnostics

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Mannose-binding lectin (MBL) deficiency caused by the variability in the MBL2 gene is responsible for the susceptibility to and severity of various infectious and autoimmune diseases. A combination of six single nucleotide polymorphisms (SNPs) has a major impact on MBL levels in circulation. The aim of this study is to design and validate a sensitive and economical method for determining MBL2 haplogenotypes. The SNaPshot assay is designed and optimized to genotype six SNPs (rs1800451, rs1800450, rs5030737, rs7095891, rs7096206, rs11003125) and is validated by comparing results with Sanger sequencing. Additionally, an algorithm for online calculation of haplogenotype combinations from the determined genotypes is developed. Three hundred and twenty-eight DNA samples from healthy individuals from the Czech population are genotyped. Minor allele frequencies (MAFs) in the Czech population are in accordance with those present in the European population. The SNaPshot assay for MBL2 genotyping is a high-throughput, cost-effective technique that can be used in further genetic-association studies or in clinical practice. Moreover, a freely available online application for the calculation of haplogenotypes from SNPs is developed within the scope of this project.

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Mannose-Binding Lectin Levels in Critically Ill Children With Severe Infections*

Cited by 5 publications

References 55 publications

Evaluation of Mannose Binding Lectin Gene Variants in Pediatric Influenza Virus-Related Critical Illness

Evaluation of Mannose Binding Lectin Gene Variants in Pediatric Influenza Virus-Related Critical Illness

Respiratory outcomes at five-year follow-up in children with MBL deficiency: a cohort study

A SNaPshot Assay for Determination of the Mannose-Binding Lectin Gene Variants and an Algorithm for Calculation of Haplogenotype Combinations

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