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3. Clinical features and risk factors for death in acute undifferentiated fever: A prospective observational study in rural community hospitals in six states of India.

Author

Mørch, Kristine, Manoharan, Anand, Chandy, Sara, Singh, Ashita, Kuriakose, Cijoy, Patil, Suvarna, Henry, Anil, Chacko, Novin, Alvarez-Uria, Gerardo, Nesaraj, Joel, Blomberg, Bjørn, Kurian, Siby, Haanshuus, Christel Gill, Antony, George Vasanthan, Langeland, Nina, and Mathai, Dilip

Subjects
RURAL hospitals, SYMPTOMS, FEVER, LONGITUDINAL method, DISEASE risk factors, DENGUE hemorrhagic fever, COMA
Abstract

Background Acute undifferentiated fever (AUF) ranges from self-limiting illness to life-threatening infections, such as sepsis, malaria, dengue, leptospirosis and rickettsioses. Similar clinical presentation challenges the clinical management. This study describes risk factors for death in patients hospitalized with AUF in India. Methods Patients aged ≥5 y admitted with fever for 2–14 d without localizing signs were included in a prospective observational study at seven hospitals in India during 2011–2012. Predictors identified by univariate analysis were analyzed by multivariate logistic regression for survival analysis. Results Mortality was 2.4% (37/1521) and 46.9% (15/32) died within 2 d. History of heart disease (p=0.013), steroid use (p=0.011), altered consciousness (p<0.0001), bleeding (p<0.0001), oliguria (p=0.020) and breathlessness (p=0.015) were predictors of death, as were reduced Glasgow coma score (p=0.005), low urinary output (p=0.004), abnormal breathing (p=0.006), abdominal tenderness (p=0.023), leucocytosis (p<0.0001) and thrombocytopenia (p=0.001) at admission. Etiology was identified in 48.6% (18/37) of fatal cases. Conclusions Bleeding, cerebral dysfunction, respiratory failure and oliguria at admission, suggestive of severe organ failure secondary to systemic infection, were predictors of death. Almost half of the patients who died, died shortly after admission, which, together with organ failure, suggests that delay in hospitalization and, consequently, delayed treatment, contribute to death from AUF. [ABSTRACT FROM AUTHOR]

Published
2023
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4. PCR based Malaria diagnostics : – Method development and application

Author

Haanshuus, Christel Gill

Subjects
parasitic diseases
Abstract

Background Almost half of the world’s population is at risk of malaria. Malaria is a parasitic vector borne disease spread by infected female Anopheles mosquitos. The protozoan parasite belongs to the genus Plasmodium group. In humans five main species are described, P. falciparum, P. vivax, P. ovale, P. malariae, and P. knowlesi. The recent years the WHO has reported that over 200 million malaria cases, and 400 000 deaths occur every year. Microscopy and rapid diagnostic tests (RDTs) are used in routine malaria diagnostics, but these methods have their challenges in accurate sensitivity and specificity. Aim To develop a new robust and user-friendly PCR method, highly sensitive and specific, and to assess and apply this method on relevant clinical material. Methods We developed a new single-step genus-specific conventional PCR targeting the cytochrome b gene (cytb) on the mitochondrial genome, and modified a species-specific conventional PCR targeting the chromosomal small subunit ribosomal RNA 18S locus. The methods were assessed and compared with routine microscopy and a gold standard nested 18S PCR using a Norwegian clinical collection (N=135), before applied in a multi-centre hospital-based study in India (N=1412). We also converted the conventional genus-specific cytb PCR to two real-time PCR assays applying SYBR Green and a TaqMan probe. The two assays were assessed using reference material, the Norwegian material (N=113) and a Tanzanian P. falciparum field collection (N= 74), and compared to five other relevant real-time PCR methods. Sequencing of the genus-specific cytb PCR products was also performed. Results Among the Norwegian sample collection (N=135) the novel genus-specific cytb PCR had a 100% sensitivity (28/28), nested 18S PCR 96% (27/28), and microscopy 93% (26/28). The 28 positive cytb PCR products were sequenced revealing six single nucleotide polymorphisms (SNPs) and one insert/deletion allowing for species determination of the 28 sequences. In the Indian multi-centre study, the cytb PCR found a malaria prevalence of 19% (268/1412). Overall, 46% P. falciparum and 38% P. vivax single infections were detected, while P. falciparum and P. vivax double infection was found in 11%, and P. malariae in 5% of the admitted fever patients. Routine microscopy and RDT had a low sensitivity compared to PCR, 29% and 24% respectively. Furthermore, the conventional cytb PCR was successfully converted to real-time PCR. The SYBR assay showed a higher sensitivity and specificity than using a probe. Focusing on detecting low-level parasitaemia, SYBR was also more beneficial to apply than probe due to melting curve analysis (MCA) can reveal unspecific binding or primer-dimers. Compared to the five other relevant real-time PCR methods our cytb SYBR PCR was the most sensitive genus-specific method. Conclusion Choice of amplification target is relevant for achieving high sensitivity in detecting low-level parasitaemia, and it is advantageous to use an intercalating fluorescence dye suitable for MCA. The highly sensitive, specific and user-friendly cytb SYBR PCR can be a useful tool in epidemiological and surveillance research, as well as for clinical malaria diagnostics. The method is genus-specific, which is an advantage in large screening projects. Among ambiguous samples, and in settings where species-specific PCR fails to detect low-level parasitaemia, confirmation and species identification by sequencing of the genus-specific real-time PCR products can be used as a contingency.

Published
2019

5. Assessment of malaria real-time PCR methods and application with focus on low-level parasitaemia.

Author

Haanshuus, Christel Gill, Mørch, Kristine, Blomberg, Bjørn, Strøm, Gro Elizabeth Ann, Langeland, Nina, Hanevik, Kurt, and Mohn, Stein Christian

Subjects
*FLUORESCENT probes, *MALARIA, *CYTOCHROME b
Abstract

In epidemiological surveys and surveillance the application of molecular tools is essential in detecting submicroscopic malaria. A genus-specific conventional cytochrome b (cytb) PCR has shown high sensitivity in field studies, detecting 70% submicroscopic malaria. The main objective of this study was to assess the conversion from conventional to real-time PCR testing both SYBR and probe protocols, and including quantitative (q) PCR. The protocols were assessed applying well-defined clinical patient material consisting of 33 positive and 80 negative samples. Sequencing of positive PCR products was performed. In addition, a sensitivity comparison of real-time PCR methods was done by including five relevant assays investigating the effect of amplification target and platform. Sensitivity was further examined using field material consisting of 111 P.falciparum positive samples from Tanzanian children (< 5 years), as well as using related patient data to assess the application of q-PCR with focus on low-level parasitaemia. Both the cytb SYBR and probe PCR protocols showed as high sensitivity and specificity as their conventional counterpart, except missing one P. malariae sample. The SYBR protocol was more sensitive and specific than using probe. Overall, choice of amplification target applied is relevant for achieving ultra-sensitivity, and using intercalating fluorescence dye rather than labelled hydrolysis probes is favourable. Application of q-PCR analysis in field projects is important for the awareness and understanding of low-level parasitaemia. For use in clinical diagnosis and epidemiological studies the highly sensitive and user-friendly cytb SYBR q-PCR method is a relevant tool. The genus-specific method has the advantage that species identification by sequencing can be performed as an alternative to species-specific PCR. [ABSTRACT FROM AUTHOR]

Published
2019
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6. A High Malaria Prevalence Identified by PCR among Patients with Acute Undifferentiated Fever in India.

Author

Haanshuus, Christel Gill, Chandy, Sara, Manoharan, Anand, Vivek, Rosario, Mathai, Dilip, Xena, Deepika, Singh, Ashita, Langeland, Nina, Blomberg, Bjørn, Vasanthan, George, Sitaram, Usha, Appasamy, Jonathan, Nesaraj, Joel, Henry, Anil, Patil, Suvarna, Alvarez-Uria, Gerardo, Armstrong, Lois, and Mørch, Kristine

Subjects
*MALARIA, *FEVER, *POLYMERASE chain reaction, *MICROSCOPY, *IMMUNITY, *PATIENTS
Abstract

Background: Approximately one million malaria cases were reported in India in 2015, based on microscopy. This study aims to assess the malaria prevalence among hospitalised fever patients in India identified by PCR, and to evaluate the performance of routine diagnostic methods. Methods: During June 2011-December 2012, patients admitted with acute undifferentiated fever to seven secondary level community hospitals in Assam (Tezpur), Bihar (Raxaul), Chhattisgarh (Mungeli), Maharashtra (Ratnagiri), Andhra Pradesh (Anantapur) and Tamil Nadu (Oddanchatram and Ambur) were included. The malaria prevalence was assessed by polymerase chain reaction (PCR), routine microscopy, and a rapid diagnostic test (RDT) with PCR as a reference method. Results: The malaria prevalence by PCR was 19% (268/1412) ranging from 6% (Oddanchatram, South India) to 35% (Ratnagiri, West India). Among malaria positive patients P. falciparum single infection was detected in 46%, while 38% had P. vivax, 11% mixed infections with P. falciparum and P. vivax, and 5% P. malariae. Compared to PCR, microscopy had sensitivity of 29% and specificity of 98%, while the RDT had sensitivity of 24% and specificity of 99%. Conclusions: High malaria prevalence was identified by PCR in this cohort. Routine diagnostic methods had low sensitivity compared to PCR. The results suggest that malaria is underdiagnosed in rural India. However, low parasitaemia controlled by immunity may constitute a proportion of PCR positive cases, which calls for awareness of the fact that other pathogens could be responsible for the febrile disease in submicroscopic malaria. [ABSTRACT FROM AUTHOR]

Published
2016
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7. Diagnosis and follow-up of treatment of latent tuberculosis; the utility of the QuantiFERON-TB Gold In-tube assay in outpatients from a tuberculosis low-endemic country.

Author

Dyrhol-Riise, Anne M., Gran, Gerd, Wentzel-Larsen, Tore, Blomberg, Bjørn, Haanshuus, Christel Gill, and Mørkve, Odd

Subjects
INTERFERONS, TUBERCULOSIS, MYCOBACTERIAL diseases, SPUTUM, TUBERCULIN test
Abstract

Background: Interferon-gamma (IFN-γ) Release Assays (IGRA) are more specific than the tuberculosis skin test (TST) in the diagnosis of latent tuberculosis (TB) infection (LTBI). We present the performance of the QuantiFERON®-TB Gold In-tube (QFT-TB) assay as diagnostic test and during follow-up of preventive TB therapy in outpatients from a TB low-endemic country. Methods: 481 persons with suspected TB infection were tested with QFT-TB. Thoracic X-ray and sputum samples were performed and a questionnaire concerning risk factors for TB was filled. Three months of isoniazid and rifampicin were given to patients with LTBI and QFT-TB tests were performed after three and 15 months. Results: The QFT-TB test was positive in 30.8% (148/481) of the total, in 66.9% (111/166) of persons with origin from a TB endemic country, in 71.4% (20/28) previously treated for TB and in 100% (15/15) of those diagnosed with active TB with no inconclusive results. The QFT-TB test was more frequently positive in those with TST ⩾ 15 mm (47.5%) compared to TST 11-14 mm (21.3%) and TST 6-10 mm (10.5%), (p < 0.001). Origin from a TB endemic country (OR 6.82, 95% CI 1.73-26.82), recent stay in a TB endemic country (OR 1.32, 95% CI 1.09-1.59), duration of TB exposure (OR 1.59, 95% CI 1.14-2.22) and previous TB disease (OR 11.60, 95% CI 2.02-66.73) were all independently associated with a positive QFT-TB test. After preventive therapy, 35/40 (87.5%) and 22/26 (84.6%) were still QFT-TB positive after three and 15 months, respectively. IFN-g responses were comparable at start (mean 6.13 IU/ml ± SD 3.99) and after three months (mean 5.65 IU/ml ± SD 3.66) and 15 months (mean 5.65 IU/ml ± SD 4.14), (p > 0.05). Conclusion: Only one third of those with suspected TB infection had a positive QFT-TB test. Recent immigration from TB endemic countries and long duration of exposure are risk factors for a positive QFT-TB test and these groups should be targeted through screening. Since most patients remained QFT-TB positive after therapy, the test should not be used to monitor the effect of preventive therapy. Prospective studies are needed in order to determine the usefulness of IGRA tests during therapy. [ABSTRACT FROM AUTHOR]

Published
2010
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8. Correction: A High Malaria Prevalence Identified by PCR among Patients with Acute Undifferentiated Fever in India.

Author

Haanshuus, Christel Gill, Chandy, Sara, Manoharan, Anand, Vivek, Rosario, Mathai, Dilip, Xena, Deepika, Singh, Ashita, Langeland, Nina, Blomberg, Bjørn, Vasanthan, George, Sitaram, Usha, Appasamy, Jonathan, Nesaraj, Joel, Henry, Anil, Patil, Suvarna, Alvarez-Uria, Gerardo, Armstrong, Lois, and Mørch, Kristine

Subjects
*MALARIA, *DISEASE prevalence, *POLYMERASE chain reaction
Published
2018
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9. Single amplification PCR targeting mitochondrial genome more sensitive in diagnosing malaria than nested 18S PCR among returned travelers in Bergen, Norway.

Author

Haanshuus, Christel Gill, Mohn, Stein Christian, Mϕrch, Kristine, Langeland, Nina, Blomberg, Bjϕrn, and Hanevik, Kurt

Subjects
*GENE amplification, *MALARIA
Abstract

An abstract of the article "Single amplification PCR targeting mitochondrial genome more sensitive in diagnosing malaria than nested 18S PCR among returned travelers in Bergen, Norway," by Christel Gill Haanshuus, Stein Christian Mohn, Nina Langeland and Kurt Hanevik is presented.

Published
2012
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