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Laboratory colonization of field Aedes aegypti
and Culex rubinotus from Uganda
Patrick P. Abila1,2,3, Bernard Bett1, Denis Mugizi1, Kristina Roesel1, Amira Al-Hosary4, Yusuf Lukenge2,
Cornelia Silaghi4, Ard M. Nijhof3
1International Livestock Research Institute; 2National Livestock Resources Research Institute; 3Freie Universität Berlin; Friedrich-Loeffler-Institute
Introduction
• Mosquito colonies are vital for investigations of both vector biology and control.
• Many mosquito arbovirus vectors have been described in Uganda
• Arboviruses, including Rift Valley fever virus are endemic in Uganda.
• Successive waves of RVF in Uganda call for better understanding of its vector biology
• No RVF competent vector colonies are being reared in Uganda.
• To this end, an insectary was established at NaLIRRI with the purpose of rearing mosquitoes
• This will improve surveillance of emerging mosquito-borne arboviruses.
Objectives
(1) To characterize laboratory rearing conditions for field colonies of A. aegypti and C. rubinotus
(2) To obtain mosquito eggs needed for RVF infection experiments at FLI
(3) To identify mosquito species collected from the field that are potential vectors of RVF
Conclusions
• Colonization of Cx. rubinotus and possibly other Culex spp. from the field requires
adjusting rearing conditions
• Nascent, local Ugandan colonies of Ae. aegypti and Cx. rubinotus for use in arbovirus
transmission studies were established.
Corresponding author: Denis Rwabiita Mugizi
d.mugizi@cgiar.org
ILRI c/o Bioversity International
P.O. Box 24384, Kampala Uganda
+256 392 081 154/155
This document is licensed for use under the Creative Commons
Attribution 4.0 International Licence. September 2022.
22 September 2022
ILRI thanks all donors and organizations which globally support its work through their contributions to the CGIAR Trust Fund.
Contribution to Uganda’s livestock development agenda
Mosquito colonies will improve the understanding of the vector biology of the mosquito
vectors of Arboviruses in Uganda.
Methodology
• A. aegypti and C. rubinotus larvae from Wakiso, Hoima, Tororo, Kampala, Mbarara, Budaka, Butebo, Napak,
Isingiro, Lyantonde, Kagadi & Rwampara were collected and incubated.
• Emerging F0 adults were offered 10% glucose solution in cotton wool for at least 4 days.
• Mosquito blood diets were drawn in EDTA from the jugular and brachial vein of a bull and hen, respectively.
• The glucose solution was withdrawn 24 hours before a blood meal.
• Blood was provided in a mosquito glass feeder or sheathed blood in collagen sausage casing.
• For the F1 of Cx. rubinotus bovine blood was spiked with glucose and fed in a glass feeder.
• Morphological identification of mosquitoes collected from RVF high risk and low risk areas is ongoing.
Biogent trap setup in Mbarara
Results
• Ae. aegypti successfully fed on both blood feeder and sausage casing while F0 of Cx. rubinotus only responded to sheathed chicken blood.
• F1 of Cx. rubinotus were able to feed on glucose spiked bovine blood in the glass feeder
• 38 filter papers with eggs of (F1= 27; F2= 7 and F3= 4) of Ae. aegypti from Hoima, Wakiso/Nakyesasa, Kampala and Tororo have been collected
• One colony of Cx. rubinotus from Mbarara is being reared and has reached F4
• All colonies from Rwampara, Budaka, Butebo, Napak, Isingiro, Kagadi and Lyantode died (the lab was still finetuning the rearing protocol)
• Morphological identification of mosquitoes from the field is ongoing
Mosquito larvae collection in Mbarara Mosquito rearing cage at NaLIRRI
Training of the team at NaLIRRI
The insectary establishedat NaLIRRI

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Laboratory colonization of field Aedes aegypti and Culex rubinotus from Uganda

  • 1. Laboratory colonization of field Aedes aegypti and Culex rubinotus from Uganda Patrick P. Abila1,2,3, Bernard Bett1, Denis Mugizi1, Kristina Roesel1, Amira Al-Hosary4, Yusuf Lukenge2, Cornelia Silaghi4, Ard M. Nijhof3 1International Livestock Research Institute; 2National Livestock Resources Research Institute; 3Freie Universität Berlin; Friedrich-Loeffler-Institute Introduction • Mosquito colonies are vital for investigations of both vector biology and control. • Many mosquito arbovirus vectors have been described in Uganda • Arboviruses, including Rift Valley fever virus are endemic in Uganda. • Successive waves of RVF in Uganda call for better understanding of its vector biology • No RVF competent vector colonies are being reared in Uganda. • To this end, an insectary was established at NaLIRRI with the purpose of rearing mosquitoes • This will improve surveillance of emerging mosquito-borne arboviruses. Objectives (1) To characterize laboratory rearing conditions for field colonies of A. aegypti and C. rubinotus (2) To obtain mosquito eggs needed for RVF infection experiments at FLI (3) To identify mosquito species collected from the field that are potential vectors of RVF Conclusions • Colonization of Cx. rubinotus and possibly other Culex spp. from the field requires adjusting rearing conditions • Nascent, local Ugandan colonies of Ae. aegypti and Cx. rubinotus for use in arbovirus transmission studies were established. Corresponding author: Denis Rwabiita Mugizi d.mugizi@cgiar.org ILRI c/o Bioversity International P.O. Box 24384, Kampala Uganda +256 392 081 154/155 This document is licensed for use under the Creative Commons Attribution 4.0 International Licence. September 2022. 22 September 2022 ILRI thanks all donors and organizations which globally support its work through their contributions to the CGIAR Trust Fund. Contribution to Uganda’s livestock development agenda Mosquito colonies will improve the understanding of the vector biology of the mosquito vectors of Arboviruses in Uganda. Methodology • A. aegypti and C. rubinotus larvae from Wakiso, Hoima, Tororo, Kampala, Mbarara, Budaka, Butebo, Napak, Isingiro, Lyantonde, Kagadi & Rwampara were collected and incubated. • Emerging F0 adults were offered 10% glucose solution in cotton wool for at least 4 days. • Mosquito blood diets were drawn in EDTA from the jugular and brachial vein of a bull and hen, respectively. • The glucose solution was withdrawn 24 hours before a blood meal. • Blood was provided in a mosquito glass feeder or sheathed blood in collagen sausage casing. • For the F1 of Cx. rubinotus bovine blood was spiked with glucose and fed in a glass feeder. • Morphological identification of mosquitoes collected from RVF high risk and low risk areas is ongoing. Biogent trap setup in Mbarara Results • Ae. aegypti successfully fed on both blood feeder and sausage casing while F0 of Cx. rubinotus only responded to sheathed chicken blood. • F1 of Cx. rubinotus were able to feed on glucose spiked bovine blood in the glass feeder • 38 filter papers with eggs of (F1= 27; F2= 7 and F3= 4) of Ae. aegypti from Hoima, Wakiso/Nakyesasa, Kampala and Tororo have been collected • One colony of Cx. rubinotus from Mbarara is being reared and has reached F4 • All colonies from Rwampara, Budaka, Butebo, Napak, Isingiro, Kagadi and Lyantode died (the lab was still finetuning the rearing protocol) • Morphological identification of mosquitoes from the field is ongoing Mosquito larvae collection in Mbarara Mosquito rearing cage at NaLIRRI Training of the team at NaLIRRI The insectary establishedat NaLIRRI